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Engine Tender

Engine Tender How does whistle on the Lionel tender car work? When you push the whistle button, what type of signal is sent? When you have no tender car, pushing the whistle button makes the engi...

 

Engine Tender

Engine Tender
How does whistle on the Lionel tender car work? When you push the whistle button, what type of signal is sent?

When you have no tender car, pushing the whistle button makes the engine run faster. However, when you have the tender, the button makes the whistle blow regardless of the speed setting, without speeding up the engine. How does this work?

...sets use a power supple that steps down the voltage from your wall outlet to a nice 16-18 volts, that is fed to the controller. The controller has a large knob to adjust the level of power to the track, and two push buttons. One button interrupts the power to the track and thus forces the the E-Unit Reversing board to cycle (if the switch on the locomotive is on...but that's a story for another day). The other button activates the horn.

The horn/whistle activation button uses diodes to place a DC pulse on top of the AC signal, the horn circuit board senses that pulse and sounds the horn.

 
Lionel 681 engine
Lionel 681 engine
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Weaver Pennsylvania Railroad SL Pacific 3768 Torpedo
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Lionel 1954 Passenger Set 2222WS W Box 2530 LgDoor
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Lionel 773 New york central hudsonCentury club 18058
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lionel midnight flyer vintageold train set 027gauge
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MTH 4106E 1 Pittsburgh Lake Erie Steam Engine
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MTH 30 1121 1 NEW YORK CENTRAL HUDSON STEAMER
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Lionel Sears 1992 Special 18024 T P 4 8 2 Mountain
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Lionel 2179WS 671RR Freight Set Original
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Lionel NYC die cast 4 4 2 steam engine whistle tender
Lionel NYC die cast 4 4 2 steam engine whistle tender
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LIONEL31778 OUTFIT 1484WS 4 CAR PULLMAN 2056 STEAMER
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MARX O guage American Locomotive w Tender 1950s Nice
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Lionel 8309 Mikado Steam Engine and Tender
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Lionel Train Engine Smoke Whistle Tender
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Marx Tin Plate 0 Gauge New York Central Train Set
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Lionel POSTWAR WHISTLING TENDER For STEAM ENGINES
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Lionel Postwar 2 6 2 K 4 No 2025 With No 6466WX Smoke
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NICE BOXED 1952 Lionel1484WS passenger set
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steam engine 224 and tender
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MTH 30 1107 2 Tone Gray Union Pacific Challenger w TMCC
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Lionel 18004 Reading Steam Engine Tender w Box C 8
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LIONEL NORTH POLE STEAM ENGINE Whistle train locomotive
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Rail King Union Pacific 4 6 2 Forty Niner Steam Engine
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LIONEL POLAR EXPRESS Engine Tender Train Car 6 28649 NB
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Lionel New York Central 2 6 4 Steam Locomotive Tender
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MTH READING 4 6 2 CRUSADER STEAMER 30 1152 0 117
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Lionel train set of tracks switches cars junk parts$
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MTH ATSF Santa Fe 2 6 0 Steam Engine
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PAYA Model Train ENGINE with COAL TENDER nib w cert NEW
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LIONEL 18056 STEAM ENGINE VANDERBILT TENDER
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WILLIAMS BRASS PENNSYLVANIA 2 10 0 LOCOMOTIVE W SOUND
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Lionel 237 engine with tender and 4 cars
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LIONEL POSTWAR PRR 681 STEAM W 2671W TENDER EXIB
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LIONEL 6 30018 PENNSYLVANIA FLYER TRAIN SET N R
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LIONEL 746 NORFOLK WESTERN WITH 746W TENDER
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On3 MMI of Precision Scale C 19 2 8 0 DRGW 342
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Marx Train Set 25249
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30S AMERICAN FLYER O GA SET BOX RUNS From Orig Owner
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MTH 2 8 2 UP USRA Mikado 20 3053 1 2535 Tender 5136
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Lionel Great Western RR General Type Steam Engine
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American Flyer 342DC Engine T Nickel Plate Road 0 8 0
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Rare Lionel 1882 General Locomotive Halloween Set
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Lionel Union Pacific 2 8 4 Berkshire Engine EXCELLENT
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Lionel Harry Potter Hogwarts Express Engine w Tender
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Lionel 646 Steam Engine and 2046W Tender
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LIONEL 1668 NEW YORK CENTAL LOCOMOTIVE AND TENDER
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LIONEL NYC 7795 STEAM ENGINE train locomotive NEW 30103
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MTH 30 1118 1 Pennsylvania RR 4 6 2 Torpedo Engine
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LIONEL 18072 1668E LIONEL LINES TORPEDO LOCO TENDER
LIONEL 18072 1668E LIONEL LINES TORPEDO LOCO TENDER
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Lionel 675 O Gauge 2 6 2 Steam Engine Tender 6466WX
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47 2025 LIONEL Locomotive Steam Engine Train Tender
47 2025 LIONEL Locomotive Steam Engine Train Tender
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Lionel New York Central 1 700E Hudson
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MTH MT 3018LP 3R O Scale Pennsylvania K 4 4 6 2 Pacific
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Lionel Postwar 1656 STEAM ENGINE BELL RINGER TENDER
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Lionel 746 Steam Loco Original box wrap No tender
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Lionel Lines Die Cast 736 Berkshire from PWC Set 31757
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Marx 2 4 2 Locomotive 666 New York Central Tender
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Lionel PostWar 4 6 4 Locomotive 2055 w tender
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Lionel Engine 2035 Original NICE Magnatraction Smoke
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Lionel Engine 675 Baldwin Wheels Smokes VERY NICE
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Marx Train Set 0 4 0 Locomotive 490 w NYC Tender
Marx Train Set 0 4 0 Locomotive 490 w NYC Tender
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1949 VINTAGE MARX ELECTRIC TRAIN
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4 4 0 General Steam Engine Union Army Gen Haupt NIB
4 4 0 General Steam Engine Union Army Gen Haupt NIB
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2 6 6 6 Imperial Allegheny Steam Engine Chesapeake Oh
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1948 Lionel 1430ws Complete Pass Train Set w Boxes NRMT
1948 Lionel 1430ws Complete Pass Train Set w Boxes NRMT
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Give your Atv Some Tender Loving Care it Deserves!

Give your ATV some tender loving care it deserves!

Everyone deserves some tender loving care from time to time, and in my opinion, so does your ATV. It has given you so much joy and excitement riding on it, so don’t you think that it’s your turn to show your ATV some tender loving care? After all, your ATV will only lasts as long as you want it to – so the more effort you put into taking care of it, the longer it lasts. Many a times, we tend to be a little careless when it comes to things like maintaining or taking proper care of our ATVs, but this attitude will have to go – IF you want to your ATV to be in tip top condition.

If you think that maintaining your ATV is a hassle, consider the hassle and trouble that you will have to go through when the parts of your ATV starts failing and you have to go all out looking for its parts – or worse, when the ATV parts that you want are not available and you have to wait for it. Waiting for your ATV parts is one thing, but missing out on the fun of ATV riding? That’s another story altogether. So, are you able to go without riding your ATV for months while you wait for those parts to arrive? No? I don’t think so too. Besides, it doesn’t have to be expensive to maintain your ATV, it may be a little time consuming but it will be even more expensive for you when you have to replace the parts of your ATV just because you were too lazy to take care of it.

So, what’s a responsible ATV owner to do then? First of all, if you love your ATV, you would want to take good care of it, so be sure that you clean up your ATV after every ride. Give it a wash after every ride and as you dry it off, be sure to check all the fasteners and levers and ride it for a minute or two to dry out the brake pads. It is also a great idea to apply WD40 to all the pivots, levers and exhaust pipe to prevent rust and premature wear and tear. To remove stubborn gasket remains and rust from exhaust pipes, I’d recommend that you try to use Scoth-Brite pads to scrub them off – yes, it works! And don’t throw away your old toothbrushes as they make good small part cleaners so you don’t have to try to squeeze your fingers into those hard to clean areas. Another great trick to keep your ATV shiny is to use some floor polish (such as Mop’n Glo) on the plastic areas of your ATV – try it and see it for yourself. It’s an inexpensive way to give your ATV that “polished” look!

Maintaining air filters regularly will make your ATV’s engine last longer and be sure to check your tire pressures for every ride, as ATV tires are inherently leaky. If you intend to ride on rocky conditions, remember to run higher tire pressures. Before every ride, always remember to check the coolant level as sometimes we are not aware that our ATV is overheated until we look into the radiator, which by then would be too late.

If you take the extra time to check and service your ATV before and after every ride, you can be sure that your ATV’s life span will be extended. Improper usage and carelessness in maintaining your ATV will only cause unnecessary damage to your ATV as well as a shorter life span. For more tips and ideas on maintaining your ATV, check out the forums at www.jackel.com or www.atvoutdoors.net - and if you have a great tip to share, by all means do so – your fellow ATV riders will thank you for it!

About the Author

For more information about kids atvs and products relating to your needs feel free to contact Jackel Motorsports toll free at 1-888-529-8629 or on the web at www.jackel.com ; www.kidatv.com ; www.atvoutdoors.com ;

Team Jackel
1-888-529-8629
http://www.jackel.com
http://www.kidatv.com
http://www.atvoutdoors.com

Scale Building

 

Scale Building

Scale Building
A student stands on a scale in an elevator at rest on the 64th floor of a building. The scale reads 844 N. ?

(a) As the elevator moves up, the scale reading increases to 917 N. Find the acceleration of the elevator.
(b) As the elevator approaches the 74th floor, the scale reading drops to 782 N. What is the acceleration of the elevator?

The long way:
F(at rest) = g * m
m = F(at rest) / g

(a) F = g(new) * ( F(at rest) / g)

F / ( F(at rest) / g)) = g(new)
917 * 9.8 / 844 = 10.65

The acceleration is = 10.65 - 9.8 = 0.85 m/s^2

(b) The elevator must be going down.
782 * 9.8 / 844 = 9.08 m/sec ^2

The acceleration is = 9.08 - 9.8 = -0.72 m/s^2

 
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Train Layout HO Scale Model Railroad 6x9
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Intermountain BNSF Maxi IV Well Cars 6 Different Sets
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HO INJECTION MOLDING PLANT w INTERIOR DETAIL 685 pcs
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100 Lot HO N Scale Train Track Power Packs Build
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HUGE LOT OF VINTAGE HO SCALE TRAIN BUILDINGS MATERIAL
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HO Scale Train Set
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How to remove Scale

Water Scales not only look bad but they can also damage your filters, pipes and their flow of pressure. Before trying to remove water scale, it is helpful to understand what water scale is. Water scale is a coating that forms on areas of the shower and taps that make contact with hard water. This hard water contains calcium or magnesium, which becomes rocklike when allowed to set. This rocklike build up can develop inside pipes and water heaters too. As a result, it can clog your pipes and cause a reduction in your water pressure. In addition, it can make your shower look grimy and dirty.

Water scale can be seen in the shower as white deposits on the shower head. It can also look like a soap film on the doors or on your tiles that is particularly difficult to remove. General spotting within the shower may also appear, making it clear that it is time to remove water scale build up. It can be difficult to remove, without proper knowledge especially if it is left for long periods of time between removals. Similar build ups can also occur within pumps, which should be removed as part of the regular maintenance.

The best method for removal is using an acid such as vinegar, by submerging the object in an acid solution for a hour or so. This works well with equipment like pumps, which can simply be placed in a bucket of vinegar solution over night. The faster that you want the scale removed the more concentrated vinegar you use. So if time isn’t a real big factor, then you can dilute it down with tap water and make the bottle of vinegar go further.
If using vinegar doesn’t remove the scale, then you need to use a stronger acid. Hydrochloric acid is perfect for the job, as it is readily available from a hardware store and will remove even the most stubborn scale in a short period of time. It may also be called muric acid. A few other agents you can use are different industrial acids, including sulfuric acid, phosphoric acid, glycine acid, and barium nitrate. These cleaners help remove water scale by breaking down the deposits left on your shower. A high pressure water jet can also help remove water scale from your shower. Care must be taken, however, when using this method to remove water scale. Otherwise, it can cause damage to the tiles or faucets of your shower.

You can always use water filters and water softeners to soften your water and keep it salt free in the first place and prevent yourself from building up of scales.

About the Author

Isopure Water carries a wide variety of point of entry filter units ranging from Water softeners, carbon filtration, and iron removal filters as well as point of use drinking water systems for residential, commercial and industrial applications. For more information visit: http://www.isopurewater.com

Wide Vision

 

Wide Vision

Wide Vision
i recently blacked out (lost vision) but apparently had my eyes wide open and i was screaming?

i had no idea i was screaming until my mom told me ...any ideas what that was? its happened to me in the past but id like to know what the term for it is.... they think it might be a seizure or just syncope so any answers are much appreciated

I have heard of a similar thing before where the person was laughing first a lot then started crying hard. It was diagnosed as a type of seizure. A visit to the doctor may be in order if it happens again.

Additional:

I've just read that you've had bad headaches and a strange sleep schedule in your questions. Try getting someone to wake you at a 'proper time early in the morning ' and getting to bed before ten at night as you wont be making serotonin which is the happy hormone and your body makes it between 8pm and 12 mn while you are sleep.

 
HO Bachmann The American Train Set 00653
HO Bachmann The American Train Set 00653
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MILWAUKEE ROAD WIDE VISION CABOOSE BY RAPIDO SUPER
MILWAUKEE ROAD WIDE VISION CABOOSE BY RAPIDO SUPER
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ATHEARN TRAINS HO DRGW SD40T 2 LOCO ROLLING STOCK
ATHEARN TRAINS HO DRGW SD40T 2 LOCO ROLLING STOCK
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Vintage Bachman HO Train Set 6 Cars More LooK
Vintage Bachman HO Train Set 6 Cars More LooK
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On30 DUNKIRK inspired conversion kit for Bachmann Locos
On30 DUNKIRK inspired conversion kit for Bachmann Locos
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Bachman 1983 Complete Train Set Unused Still in Boxes
Bachman 1983 Complete Train Set Unused Still in Boxes
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Rapido Trains 110023 Wide Vision Caboose Chessie
Rapido Trains 110023 Wide Vision Caboose Chessie
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Overland Limited Train Set By Bacmann
Overland Limited Train Set By Bacmann
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NEW HO Transcona Ontario Northland Lighted Caboose 126
NEW HO Transcona Ontario Northland Lighted Caboose 126
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Athearn RTR F7A B Canadian National CN Stewart Chassis
Athearn RTR F7A B Canadian National CN Stewart Chassis
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NIB HO Walthers 931 700 GP9 Alaska 1802 w Caboose
NIB HO Walthers 931 700 GP9 Alaska 1802 w Caboose
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HO Scale MOHAWK 4 8 2 NYC STEAM FREIGHT SOUND DCC MTH
HO Scale MOHAWK 4 8 2 NYC STEAM FREIGHT SOUND DCC MTH
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Bachmann 502 HO DCC SET STEAM DIGITAL COMMNDR UP
Bachmann 502 HO DCC SET STEAM DIGITAL COMMNDR UP
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Bachmann SANTA FE Digital Commander Train Set 501
Bachmann SANTA FE Digital Commander Train Set 501
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NEW ONTARIO NORTHLAND wide vision caboose
NEW ONTARIO NORTHLAND wide vision caboose
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Bachmann HO Thoroughbred Train Set 691 NIB Bachman H O
Bachmann HO Thoroughbred Train Set 691 NIB Bachman H O
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MTH 80 3123 1 HO 4 8 2 L 3a Mohawk NYC 3006 DCC Sound
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BAC00647 HO Scale Santa Fe Flyer Train Set Brand New
BAC00647 HO Scale Santa Fe Flyer Train Set Brand New
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MTH 80 3123 1 NYC L 3a 4 8 2 Mohawk Steam Brand New
MTH 80 3123 1 NYC L 3a 4 8 2 Mohawk Steam Brand New
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HO TRAINS CHALLENGER UNION PACIFIC COMPLETE TRAIN SET
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BAC691 Thoroughbred Train Set Bachmann
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BACHMANN 00621 CHALLENGER READY TO RUN TRAIN SET SEALED
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MTH New York Central NYC 4 8 2 L 4b Mohawk 3125 NEW
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New York Central L3 A Mohawk 4 8 2 Steam Engine 3006
New York Central L3 A Mohawk 4 8 2 Steam Engine 3006
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NIB HO Bachmann 647 Santa Fe Flyer Train Set
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BACHMANN HO 647 HO Santa Fe Flyer Set FT Diesel MIB
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HO JOHN DEERE 1997 MINT LIMITED JD TRAIN SET FIRST SET
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HO SCALE TRAINS SANTA FE FLYER COMPLETE TRAIN SET NIB
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Rapido Trains 110051 Wide Vision Caboose NP
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Rapido Trains 110043 Wide Vision Caboose Milwaukee
Rapido Trains 110043 Wide Vision Caboose Milwaukee
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Rapido Trains 110047 Wide Vision Caboose Milwaukee
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BAC647 Santa Fe Flyer Electric Train Set by Bachmann
BAC647 Santa Fe Flyer Electric Train Set by Bachmann
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BAC614 Overland Limited Train Set by Bachmann
BAC614 Overland Limited Train Set by Bachmann
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HO BRASS OMI FRISCO WIDE VISION CABOOSE CUSTOM PAINTED
HO BRASS OMI FRISCO WIDE VISION CABOOSE CUSTOM PAINTED
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Bachmann 691 HO THOROUGHBRED FREIGHT SET
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NIB HO Rapido TY 110064 WV Caboose RI 17017
NIB HO Rapido TY 110064 WV Caboose RI 17017
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NIB HO Rapido TY 110045 WV Caboose Milw Rd 992303
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Athearn HO SCALE 79675 GP40 2 CHESSIE BO 4103 EXTRAS
Athearn HO SCALE 79675 GP40 2 CHESSIE BO 4103 EXTRAS
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Walthers Limited Edition CENTURY 21 8 Unit Train Set
Walthers Limited Edition CENTURY 21 8 Unit Train Set
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Athearn HO BO Baltimore Ohio SW 7 Diesel Switcher Set
Athearn HO BO Baltimore Ohio SW 7 Diesel Switcher Set
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Athearn RARE CABOOSES of MEXICO NdeMFCPSet HO Train
Athearn RARE CABOOSES of MEXICO NdeMFCPSet HO Train
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Bachmann 00637 The American HO Train set MIB
Bachmann 00637 The American HO Train set MIB
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Bachmann 00647 Santa Fe Flyer Set HO
Bachmann 00647 Santa Fe Flyer Set HO
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Model Power Twin Diesel Set HO
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Bachman Sante Fe Flyer HO Train Set
Bachman Sante Fe Flyer HO Train Set
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Bachmann 00621 Challenger Set HO Exclusive
Bachmann 00621 Challenger Set HO Exclusive
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BACHMANN HO COMPLETE R T R KDs ELECTRIC TRAIN SET
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Bachmann Digital Commander RTR Electric Train Set 501
Bachmann Digital Commander RTR Electric Train Set 501
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HO Scale Santa Fe Flyer Train Set SF Santa Fe
HO Scale Santa Fe Flyer Train Set SF Santa Fe
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MTH 80 3127 1 HO 4 8 2 L 4b Mohawk NYC 3125 DCC Sound
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Bachmann HO Overland Limited Union Pacific 9 cars
Bachmann HO Overland Limited Union Pacific 9 cars
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Bachmann 614 Overland Limited Union Pacific UP Freight
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Rapido ONTARIO NORTHLAND WV Caboose 122 w Lights NIB
Rapido ONTARIO NORTHLAND WV Caboose 122 w Lights NIB
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Bachmann Union Pacific Overland Limited with Nine cars
Bachmann Union Pacific Overland Limited with Nine cars
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Rapido Trains 110065 Wide Vision Caboose RI
Rapido Trains 110065 Wide Vision Caboose RI
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Bachmann HO 00691 Norfolk Southern Thoroughbred Set
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Bachmann HO 00501 SF Digital Commander DCC Starter Set
Bachmann HO 00501 SF Digital Commander DCC Starter Set
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New HO DCC DIESEL DIGITAL COMMANDER Set by Bachman
New HO DCC DIESEL DIGITAL COMMANDER Set by Bachman
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Bachmann HO Scale Santa Fe Flyer Train Set 00647
Bachmann HO Scale Santa Fe Flyer Train Set 00647
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Vision, Mission, Purpose: What Does it All Mean?

We hear the words purpose, vision and mission everyday, but what do they really mean and how are they different from each other? It is easy to puzzle over these questions for hours. Large companies will pay consultants tens of thousands of dollars to help them craft elegant statements to adorn their walls and motivate their employees. Many times these become so overlaid with business jargon that they end up not saying much at all. As a small business, choosing the right words and applying them to your business can serve the organization by defining leadership roles, unifying efforts, setting departmental and company-wide goals, better serving customers and encouraging and motivating employees. However, the larger purpose of defining these words and applying their meaning is to illuminate your focused strategy and ensure that everyone that comes in contact with your company has a clear understanding of what your organization is abut and what they can rely on you for. A few well crafted sentences can save a tremendous amount of time in the long run, by becoming crystal clear on the answer to – What are we here for?

First you must be able to see your vision. Companies like many things in our universe start as nothing but an idea in someone’s mind and then turn into a physical reality. In order to get others actively working towards creating that physical reality, they must be able to see the vision; therefore, you must be able to convey it. A business’s vision is a desired future. It can help to guide all who accept and understand it. A shared vision can be a great tool for building a sense of belonging and community. A vision is not a CEO’s desire to make a billion dollars. While a CEO’s ideas are important to the future of the company, the management team and other players’ are equally as important because they relate to personal commitment to the business. If employees don’t believe in a company they are less likely to give their best effort. The old adage, ‘You are only as strong as your weakest link’ can be very true. The questions you need to ask in order to frame your vision are, “What value do we offer the market?†and “How are we going to offer it in a unique way?†Unlike a company’s goals but similar to its mission, a vision does not have a deadline. It can evolve with the company and can be vague or exact to have impact and meaning. A company’s vision is how it sees itself fitting into the marketplace at large. Think of your vision as your “I have a dream speech†for your business.

Next we define the mission and the purpose. Sometimes the mission and the purpose are the same thing, and other times it is worth separating them. A company’s Mission Statement defines why your organization exists; the purpose gets into what it hopes to achieve in the future and how they fit into the greater good of society and the world. Your mission answers the question “What are we here to do?†It should be well defined, so it can guide your business’ planned actions.

A company’s purpose answers the question, “Why do our mission and vision matter?†That can include giving back to employees, management and shareholders. Some company’s say their purpose is to serve all related parties from workers to clients in the best way possible. Others are in existence solely to make money. There is no right or wrong purpose. There is only what you decide your organization is meant to do. The dictionary says that a purpose is “an anticipated outcome that is intended or that guides your planned actions.†This anticipated outcome can be spiritual, practical or comical. It can be health or environmentally conscious or convenience oriented. It is how ever you see your organization changing the world, in whatever small or big way you intend to.

For example, the mission of a bicycle part manufacturing company could be to make the highest quality bicycle parts that allow customers to maximize the usable life of their bike. Or it could be to be the largest bike part manufacturer in the world or to be the brand of choice for cost conscious customers or to be the trusted vendor of the largest athletic chain stores. Their purpose may be to make solid, safe parts to improve bike safety, or to make a community or an entire planet healthier by encouraging outdoor bike riding as a form of exercise, or to encourage people to use bikes as transportation rather than cars an reduce pollution. You can see how these different missions and purposes would guide a company to operate in different ways.

When Mark Walker decided to re-brand his business J M Walker Group with a mind for building a solid, valuable entity for the future, that he could pass on to his children one day, he wanted to make sure he built on a strong foundation. He started by defining his vision, mission and purpose with the following:

Vision (What this business means to me): To empower companies and individuals rise to their highest potential through high quality training content and inspiring delivery.

Mission (What we are here to accomplish): To be a premiere provider of training to large and mid-size companies in the Southeast. We help businesses grow value and profits by training their people to become exceptional in selling, serving, communicating and managing time, with clients, customers and their daily contacts. We get excited when people tell us that they feel like they are now part of something bigger than themselves, and see great value in what they do to serve their customers, clients, or patients.

Purpose (What my business means to the world): The purpose of J M Walker Group is to leave a legacy of earning an excellent living, using and sharing our gifts and talents to help businesses and individuals succeed. We desire to bring a positive view of God to our marketplace and to reflect His special love for people in all that we do.

Once you get the right vision, mission and purpose on paper, you can then move on to setting meaningful goals to move the business forward in those directions.

It is important for any organization to spend time figuring out what their purpose, vision and mission are so that all parties involve to understand them implicitly. This insures that everyone is moving in the same direction, which is critically important for being able to grow quickly. Taking the necessary time to assess these three words is critical because a company should be a machine with many differentiated parts, but only one mind. For more information on how you can improve your business, visit www.flourishingbusiness.com.

About the Author

Elizabeth W. Gordon, founder and President of The Flourishing Business, LLC, is a visionary leader who has a passion for helping others achieve their entrepreneurial dreams and enjoy more of the best in life. With a vast and diverse background in many business arenas, Elizabeth regularly has the opportunity to share her business acumen with clients, large and small. She currently serves on the Board of Directors of the National Association of Women Business Owners (NAWBO), Atlanta and the Board of Directors of the American Association of University Women (AAUW) Atlanta. She is an Accredited Executive Associate of the Institute for Independent Business (IIB) and a certified Life Coach.

Lamp Post

 

Lamp Post

Lamp Post
Am I crazy or was there a song and about a man falling in love with a lamp post?

I'm sure it wasn't a dream but I distinctly remember a music where a man fell in love with a lamp post, he even cuddled it in bed at one point. Nobody believes me!

Lovestruck by Madness. It has a line about falling for a lamp post in the chorus.

 
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250WHITE LED E10 DC12V BULB LIGHT LAMP for LIONEL MARX
250WHITE LED E10 DC12V BULB LIGHT LAMP for LIONEL MARX
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500 WHITE LED BA9S T4W 182 12V GLOBE BULB LIGHT LAMP
500 WHITE LED BA9S T4W 182 12V GLOBE BULB LIGHT LAMP
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500WHITE LED E10 12V BULB LIGHT LAMP for LIONEL MARX
500WHITE LED E10 12V BULB LIGHT LAMP for LIONEL MARX
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250WHITE LED E10 12V BULB LIGHT LAMP for LIONEL MARX
250WHITE LED E10 12V BULB LIGHT LAMP for LIONEL MARX
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250 WHITE LED BA9S T4W 182 12V GLOBE BULB LIGHT LAMP
250 WHITE LED BA9S T4W 182 12V GLOBE BULB LIGHT LAMP
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LIONEL 6357 SOUTHERN PACIFIC ILLUMINATED CABOOSE OB
LIONEL 6357 SOUTHERN PACIFIC ILLUMINATED CABOOSE OB
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LIONEL PW 395 FLOODLIGHT TOWER 4 LIGHTS IT WORKS
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LIONEL TRAINS POSTWAR 70 LAMP POST O BOX
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500 WHITE BA9S T4W 12V LED GLOBE BULB LIGHT for LIONEL
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MTH Train No 64 1930s Lamp Post Set 30 11003 Black MIB
MTH Train No 64 1930s Lamp Post Set 30 11003 Black MIB
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LIONEL TRAINS POST WAR 456 DARK GREY COAL RAMP CONTROL
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500White E10 12V Led Bulb Light Lamp for DIY LIONEL
500White E10 12V Led Bulb Light Lamp for DIY LIONEL
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CS 2 O Scale Crossing Signal Set for Lionel MTH Atlas
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LIONEL POST WAR TRAIN SET 5 CARS POSTWAR GREAT SHAPE
LIONEL POST WAR TRAIN SET 5 CARS POSTWAR GREAT SHAPE
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LIONEL 6419 DL W WRECKING CAR VG EX
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Lionel 58 Lamp Post Cream Color
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Lionel 0 27 NY Central Flyer Train Set 6 11735 EXTRAS
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Citgo Animated Billboard Sign 0 or H0 size
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LIONEL POSTWAR 1958 52 FIRE CAR MOTORIZED UNIT EX RARE
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3 Traffic Lights for Vintage USSR Electrical Train Set
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100 50WL20RL 10YL10GL10BL 12V E10 Led Bulb Lamp
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LIONEL POSTWAR 71 LAMP POST SET OF FOUR
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Electrical RAILROAD Train SET 1960s Extremely RARE
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RARE LIONEL PREWAR 922 COPPER LAMP 56 TERRACE PLOT
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Aristo Craft O or S Brass Street Lamps Box of 4
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Bing O gauge Wind cutter 0 4 0 20vElec VG but no tender
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8 Chicago Line 37 Boulevard Light 35 Crown Of Thorns
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Lionel Train Set 1926 Standard Gauge
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Built O Scale Art Deco VFW Post from Trackmun
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How to Install an Outdoor Post Lighting System

There are many ways you can use to decorate the exteriors of the house. One of the most brilliant ideas is to use post lighting to heighten the beauty of your house.

Decorative lighting is a method of decorating by using light and light effects. You can use various techniques like patios, fountain lighting, steps lighting, silhouetting, shadowing. But the outdoor post lighting gives your house the much sought after regal look. This helps to create a pleasant amicable atmosphere for conducting outdoor activities. If the lights are used creatively it can create a good mood that can add a feather to the arrangements. Those having lawns, drive ways, and gardens certainly need post lighting. This has twofold use; one is aesthetic purpose and another is safety purpose. Use of creative ability and imagination are the driving force behind such beautiful lightings.

These outdoor post lightings are powered by low voltage lighting system. The use of low voltage systems amount to an economical use of power resources. If you use lantern instead of lamps it creates a nice atmosphere. These lamps usually work on citronella oil and can keep mosquitoes away.

The light decoration of exteriors has evolved into an art form. There is vast range of outdoor post lighting and are based on the energy saver low voltage system. The system needs merely a current of 12 volts. This needs a transformer which converts 120 volt current to 12 volt current. Just check whether the transformer can provide enough wattage to support more lights. These systems are easy to operate.

There are certain precautions that to be taken for outdoor post lighting. Check whether the lights are tested by recognized laboratory. Always select a fuse plugged light, replace burned out plugs, and check for cracked sockets. Loose connections and bare wires can be hazardous. It is important to make sure that the lights you are using are intended for outside use.

The outdoor post lighting helps you to illuminate the road to home properly. These lights are specially designed to withstand conditions like typhoons, hails, and rain. These adverse conditions do not have any effect on post lightings.

The most economical and convenient way is to install solar powered post lighting. It is easily available in stores. These lamps do not need any kind of installation and are charged by sunlight. This energy suffices to keep the light shining throughout the night. There are many energy saver bulbs which you can use in lieu of normal bulbs.

There are many varieties of lamp post which are superb in style. These posts give an ambient glow to the house. These posts can be easily situated as per the requirements. You can set them on the side of the curb to welcome the guests or can set in the backyard at time of entertainment activities. The lamp posts are available in lantern style in various finishes. The bronze finish, sepia finish, verbena finish, terra finish, silver finish, brimstone finish are some of the quite exquisite varieties. The post lanterns are also available in umpteen varieties. They are also made up of various materials and are available in different finishes.

About the Author

Muna wa Wanjiru Has Been Researching and Reporting on Outdoor Lighting For Years. For More Information on Outdoor Post Lighting, Visit His Site at

Scale Building

 

Scale Building

Scale Building
Does anyone have plans on building a display case for HO scale train cars and locomotives?

My friend is an avid HO scale railroad modeler. He has an extensive collection of locomotives and cars that in some cases are quite beautiful and would look nice in a display case. I'm looking for simple plans that will provide an opportunity for him to display and protect his investment.

im sure he has "model railroader" ...its a magazine

 
Silver Rail Express Battery operated Train Set
Silver Rail Express Battery operated Train Set
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MTH 30 2125 1 Delaware and Hudson PA 1 AA Diesel Set
MTH 30 2125 1 Delaware and Hudson PA 1 AA Diesel Set
Paypal   US $60.99
Walthers 2707 O Scale Golden Valley Depot Built Up
Walthers 2707 O Scale Golden Valley Depot Built Up
Paypal   US $59.50
Walthers 3304 O Scale Kit Phoenix Fuel Oil Corp
Walthers 3304 O Scale Kit Phoenix Fuel Oil Corp
Paypal   US $59.50
Walthers 3312 O Scale O 27 Kit Krazy Kens Car Town
Walthers 3312 O Scale O 27 Kit Krazy Kens Car Town
Paypal   US $64.50
O 148 MANAGERS COTTAGE KIT for Mine or Mill
O 148 MANAGERS COTTAGE KIT for Mine or Mill
Paypal   US $58.94
O Scale Scratch BUILT Not Kit CUSTOM Building On3 On30
O Scale Scratch BUILT Not Kit CUSTOM Building On3 On30
Paypal   US $75.00
Walthers 2707 O Scale Golden Valley Depot NEW
Walthers 2707 O Scale Golden Valley Depot NEW
Paypal   US $35.00
MTH 20 66122 Amtrak 2 Car SuperLiner Coach Set
MTH 20 66122 Amtrak 2 Car SuperLiner Coach Set
Paypal   US $216.99
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MTH 30 2513 1 PCC Pacific Electric Street Car
Paypal   US $113.99
O scale On30 On3 scratch Built Structure Building 14
O scale On30 On3 scratch Built Structure Building 14
Paypal   US $50.99
Lionel 6 18007 Southern Pacific Daylight Steam Engine
Lionel 6 18007 Southern Pacific Daylight Steam Engine
Paypal   US $121.50
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Lionel 6 18009 NYC L3 Mohawk Steam Engine Railsounds
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Lionel 6 18043 CO Streamlined Hudson Steam Engine TMCC
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Lionel 6 18563 NYC 2380 GP 9 Diesel Engine TMCC RS
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Lionel 6 8406 NYC Scale Hudson Steam Engine 783
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Lionel Post War 2339 Wabash GP 7 Diesel Engine
Lionel Post War 2339 Wabash GP 7 Diesel Engine
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Lionel Post War 2530 Aluminum REA Baggage Passenger Car
Lionel Post War 2530 Aluminum REA Baggage Passenger Car
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Lionel PW 2033 Union Pacific AA Alco Diesel Engines
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Lionel Southern Pacific FM Trainmaster Diesel Engine
Lionel Southern Pacific FM Trainmaster Diesel Engine
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Lionel Lackawanna Smooth Aluminum 6 Car Passenger Set
Lionel Lackawanna Smooth Aluminum 6 Car Passenger Set
Paypal   US $78.00
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Lionel 6 18583 AEC 57 Postwar Celebration Switcher EX
Paypal   US $105.50
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MTH 20 3125 1 SP AC 6 4 8 8 2 Cab Forward Steam Loco
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IVES 115 Freight Station 1920s GREEN BUILDING O Scale
IVES 115 Freight Station 1920s GREEN BUILDING O Scale
Paypal   US $49.95
Lionel 6 18583 AEC 57 Postwar Celebration Switcher MT
Lionel 6 18583 AEC 57 Postwar Celebration Switcher MT
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MTH 30 9101 Sinclair Operating Gas Station NIB
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K Line 6 22140 CNJ Boxcab Diesel Locomotive w Horn EX
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MTH 30 11028 Wood Water Tower LN Box
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MTH 30 9106 Esso Operating Gas Station NIB
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O On30 148 Large Corrugated Iron BUSH STRUCTURE KIT
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Korber Models 969 General Lt Pwr Office O Scale NEW
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Lionel SD 40 2 CSX Husky Stack Diesel Freight set
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Stoney Creek Designs Hodges Pharmacy Kit O On3 On30
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O On3 On30 STONEY CREEK DESIGNS 9 A BLOCK OF BUILDINGS
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o scale granary Lionel MTH buildings structures
o scale granary Lionel MTH buildings structures
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K Line Mainline PINE VALLEY LOGGING COMPANY NIB
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THROPTONS FURNITURE COMBO O Model Railroad Structure
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BO HOTEL O On30 Railroad Board on Laser Structure Kit
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BLACKSMITH CARPENTER SHOP Railroad Structure Kit O On30
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COLORADO SOUTHERN RAILROAD SILVER PLUME BAKERY O On30
COLORADO SOUTHERN RAILROAD SILVER PLUME BAKERY O On30
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30 40s ERA GAS STATION O Model Railroad Structure Kit
30 40s ERA GAS STATION O Model Railroad Structure Kit
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DRGW STOCK PENS Model Railroad Structure Kit O On30
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RIO GRANDE SOUTHERN RAILROAD OPHIR DEPOT O On30 Kit
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LITTLE CREEK ENGINE HOUSE Model Railroad Kit O On3 On30
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COLORADO SOUTHERN RAILROAD SILVER PLUME HOUSE O On30
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RGS OILTON SALOON O On30 Model Railroad Structure Kit
RGS OILTON SALOON O On30 Model Railroad Structure Kit
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TRAILWAYS BUS STATION BUS STATION DOCK
TRAILWAYS BUS STATION BUS STATION DOCK
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O Scale Brass PONY TRUSS BRIDGE
O Scale Brass PONY TRUSS BRIDGE
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Lionel Prewar 1688 EngineTenderTrackBiuldingsSigns
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MTH RailKing AW Rootbeer Fast Food Restaurant Stand
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MTH 30 90298 Country Store Railtown General Store
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Lionel Neils Guitar Shop 6 16883
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WALTHERS O 027 BACK GROUND BULDING SET OF 2
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Lionel 6 62162 Operating Crossing Gate Signal
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GEO WICKETT FEED AND SEED SCHOMBERGFREE SHIPPING
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Atlas O 0607 1 40 CP Rail Stock Car 3 rail Std O NIB
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MTH Country Passenger Depot Lighted Maroon Cream NEW
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MTH DCS Accessory Interface Unit AIU 50 1004 Sealed
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Konrad Paint Co O Scale
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Heier Kite Co O Scale
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Birdies Tavern O Scale
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O Cornerstone Preassembled Silver Dollar Cafe 2712
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MTH 30 90325 Pittsburgh Steelers 193 Water Tower
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MTH Railking NYC Proto 20 Switcher Diesel Engine 2217
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O RURAL VALLEY DEPOT CREAM n GREEN ASSEMBLED BUILT
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Yorke Ace Coal Company Plaster Resin kit O On3 On30
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MTH 40 750C Railking Hobby Transformer Controller Set
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ENCOURAGING THE FUTURE WITH GREEN BUILDING

ENCOURAGING THE FUTURE WITH GREEN BUILDING

By Kaushik K. Shandilya

Legionnaires' outbreak incidents were regularly reported from a 1976 Philadelphia convention at the Bellevue Stratford Hotel and the Croatia Hotel. The source of the bacteria was contaminated water used to cool the air in the hotel's air conditioning system. Moreover, people dream of living long into their seventies, eighties or even nineties. Both these causes and incidents certainly indicate the effect of bad indoor air quality on human life. Sometimes living healthy does not take strict dieting or excessive exercise,  but the right place to live. This is why green building is ideal for people who care about good-quality living, an important issue in recent times. Unfortunately, only a few middle- or upper-class urban and suburban residents trust or even know about advantages of healthy environment of green buildings.

Conventionally, the houses we live in are often made from wood or concrete, which cause some dilemmas and adversities. Green building practices tend to decrease the environmental impact of buildings. Buildings account for a large quantity of land use, power and water consumption, and air and atmosphere shift. Typically, buildings use slightly less than half of the total power and one eighth of the total amount of water consumed in both the U.S. and the European Union.

The poor building quality issue is not just about atmosphere: individuals are harmed too. For example, a typical American or European spends 90 percent of his or her time indoors, which is at least twice as contaminated as outdoor air. Mortality and morbidity associated with this is well established in scientific literature. Indoor air quality also causes financial stress as health and productivity losses cost tens of billions of dollars annually to the nation. Buildings liberate large amounts of particulate matter and sulfur dioxide and produce raw building materials. While particulate matter and sulfur dioxide are detrimental to human health, the raw building materials and debris cause solid waste management problems and global warming.

Green building avoids the conventional construction pitfalls and provides residents with a good, healthy indoor environment. Green building brings together an infinite range of practices and techniques to decrease and eliminate the impacts of buildings on the environment and human health. The innovations of green building and inside-building are increasing day by day. The Rocky Mountains Institute in Colorado includes a green building interior garden which fosters bananas, orange trees, lizards, avocados, grapes, papayas and passion fruit—even in the mountains at 104ºF. Building materials usually considered to be 'green' comprise renewable plant materials like bamboo (as bamboo grows rapidly) and straw, lumber from forests, dimension and recycled stone, recycled metal and other products that are safe, reusable, renewable and/or eco-friendly (e.g. linoleum, sheep wool, panels made from paper flakes, adobe, compressed, baked and rammed earth, clay, vermiculite, sea grass, cork, coconut, wood fiber plates, calcium sand stone, high and ultra high performance concrete, etc).

The ING Bank Building in Amsterdam is also a superior example of the positive benefits of green building. It is an organic building with natural materials, natural light and interior gardens with small waterfalls. Natural ventilation through operable windows is used in place of air conditioning. A cogeneration system powers an absorption chiller by waste heat for dehumidification. The 1500 USD cost is cheaper than for many banks which consume five times as much energy. Green buildings frequently comprise measures to reduce energy use. To enhance the effectiveness of the building envelope, they may employ high-efficiency windows and insulation in walls, ceilings and floors. Moreover, efficient window position (day lighting) can offer natural light and reduce the need for electric lighting. In conclusion, onsite creation of renewable energy through solar power, wind power, hydro power or biomass can notably decrease the environmental impact of the building.

It often emphasizes taking benefit of renewable resources, e.g., using sunlight through passive and active solar, and using vegetation through green roofs, rain gardens and for decrease of rainwater run-off. Other interesting techniques, such as packed gravel for parking lots as a substitute of concrete or asphalt to enhance percolation of ground water, are used as well. The Queen's Building at De Montfort University, Leicester’s the biggest naturally ventilated building in the U.K.  Most shell area is operable so the occupants can operate windows to regulate their comfort conditions. Air flows throughout the building by means of chimney effect.  Heating is accomplished by the use of passive solar and internal heat gain from the occupants and equipment. In fact, a collection of smaller domestic scale buildings, the huge masonry structure has gorgeous polychromatic brickwork by local masons and offers the thermal mass for the structure. Carefully designed overhangs and a narrow footprint permit sunlight in during the cooler months and blocks it during the heat of summer. The classrooms in this superior building have natural day lighting and require virtually no powered lighting.

Green architecture also seeks to trim down waste of power, water and materials used during construction. In the construction phase, one goal is to decrease the material going to landfills. Well-designed buildings also assist to decrease the waste generated by the occupants as well, by offering such onsite solutions as compost bins to reduce matter going to landfills. The Passivhaus in Darmstadt, Germany uses only 10 percent of the energy required by other houses in the city and only 25 percent of the typical electrical energy. Rather than being gloomy and repressive as might have been the case, the Passivhaus is dazzling and cheerful and very much linked to nature.

By collecting human waste at the source and running it to a centralized biogas plant with biological waste, fertilizer can be produced. This idea was verified by a resolution in Lubeck Germany in the late 1990s. Practices like these make available soil with organic nutrients and create carbon sinks that eliminate CO2 from the atmosphere, offsetting GHG emission. Producing synthetic fertilizer is also costlier in energy than this process.

Why is green building not used more often? The answer rests in fears and assumptions made overtime by decision-makers in the building industry. The environmental impact of buildings is underestimated, while the apparent costs of green buildings are overestimated. A recent investigation by the World Business Council for Sustainable Development finds that green expenses are overrated by 300 percent. Some property holders don’t take the time to research the benefits of green building. Some lack knowledge and experience in construction and depend too much on older technology and regulations, without regard to the quality which it often lacks. Quick assumptions also abound among lenders and funders afraid of the cost risk. They may think that since wood and concrete are so profitable, they should not give them up.

Apparently, it doesn’t matter to the holders that green buildings produce greater benefits in health, well-being and productivity (thanks to day-lighting). Resource consumption is minimized, construction waste is low, resource reuse is maximized, the natural environment is better protected, energy efficiency is greater and human health is improved thanks to the absence of toxics. Those who care about this quality of living should carefully compare green building with the more common but inferior buildings available. They may be surprised by the healthier lifestyle that comes from green building. According to U.S. EPA, reducing the amount of natural resources buildings consume and the amount of pollution caused is crucial for future sustainability.

About the Author

Kaushik K. Shandilya is a Civil Engineering graduate student and a member of the University of Toledo AWMA student chapter.

Engine Tender

 

Engine Tender

Engine Tender
please help me girls...?

Earlier today I was playing with my train set, when things took a turn for the worse. One of the small plastic buildings got stuck in my bottom and I didnt know what to do. Normally if it was real life, I would call the fire department. Applying this knowledge to the situation at hand, I sent in my toy fire engine and now it is stuck as well. Now logically the army is the next step but I am a little nervous about all those tin soldiers and the area is now a little tender.
Maybe a nice young lady would accompany me to the doctors so it doesent look so bad, and maybe we will fall in love with each other.

LMAO! The next step would actually be to call a tow truck,but I don't think that's wise in your situation either! Yes,better go to the docs right away and stop playing with the the toys that way!

 
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HO Brass Hallmark ATSF 4 8 4 3752 f p new
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BACHMANN HO NEW YORK CENTRAL NIAGRA POWERED LOCOMOTIVE
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HO Brass Challenger Imp 22781 N 3 Milw 2 6 6 2 Mint
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HO Brass WR Northern Pacific S 4 4 6 0 Version 2 Mint
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Marklin HO Steam Locomotive Tender DB BR 24 3003
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HO Model Loco DJH ML238 BR 3482 wurtt Ac 2 4 0
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NEW Mantua HO Pacific W Steam Sound Crescent Lmt NIB
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BRASS NPP READING 2 8 2 M 1sa UNPAINTED MINT
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ALCO DIESEL GT MIB GG1 PENN DIESEL MIB 13 MORE MIB
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Fleischmann Tender loco of the DRG class 3810 40 Dig
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HO Scale VT Old Timer Steam Locomotive Set Bachman
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Bachmann Spectrum Santa Fe Baldwin 2 8 0 DCC Sound HO
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BRASS CHICAGOBURLINGTON QUINCY CBQ CLASS O5B CP
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Custom Athearn Genesis Santa Fe 2 8 2 Light Mikado DCC
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John Bull HO Train Engine Tender 3 cars
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BRASS CHICAGO BURLINGTON QUINCY 2 10 4 PRO PAINT
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Rivarossi HO 4 6 4 New York Central Engine EXC 5446
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BACHMANN HO HARRY POTTER HOGWARTS EXPRESS TRAIN SET
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BACHMANN HO OVERLAND LIMITED STEAM ERA BOXED TRAIN SET
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HO BRASS NYC 4 8 2 MOHAWK LMBLUM KTM OF JAPAN
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Lima HO Scale Engine 3008L
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Wrenn HO W2226 Locomotive Tender NMIB City of London
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BRASS PSC BOO RIM DRGW 2 8 8 2 L 131 F P GREEN BOILER
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DIVISION POINT DP 8196 KCS J CLASS STEAM FLAG RARE
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Future prospects of enzyme engineering and enzyme technology

Future prospects of enzyme engineering

Enzyme engineering is the recent technology growing rapidly due to its higher application in a lot of fields and due to having bright and clear future vision. A most exciting development over the last few years is the application of genetic engineering techniques to enzyme technology. There are a number of properties which may be improved or altered by genetic engineering including the yield and kinetics of the enzyme, the ease of downstream processing and various safety aspects. Enzymes from dangerous or unapproved microorganisms and from slow-growing or limited plant or animal tissue may be cloned into safe high-production microorganisms. The amount of enzyme produced by a microorganism may be increased by increasing the number of gene copies that code for it. For example; The engineered cells, aided by the plasmid amplification at around 50 copies per cell, produce penicillin – G – Amidase constitutively and in considerably higher quantities than does the fully induced parental strain. Such increased yields are economically relevant not just for the increased volumetric productivity but also because of reduced downstream processing costs, the resulting crude enzyme being that much purer. New enzyme structures may be designed and produced in order to improve on existing enzymes or create new activities. Much protein engineering has been directed at Subtilisin (from Bacillus amyloliquefaciens), the principal enzyme in the detergent enzyme preparation, Alcalase. This has been aimed at the improvement of its activity in detergents by stabilizing it at even higher temperatures, pH and oxidant strength. A number of possibilities now exist for the construction of artificial enzymes. These are generally synthetic polymers or oligomers with enzyme-like activities, often called synzymes. Enzymes can be immobilized i.e., an enzyme can be linked to an inert support material without loss of activity which facilitates reuse and recycling of the enzyme.Use of engineered enzyme to form biosensor for the analytical use is also recent activity among the developed countries. Some enzymes make use in diseases diagnosis so they can be genetically engineered to make the task easier. Thus it is obvious that there is huge scope of the enzyme technology in the future as well as in present.

Introduction

Enzymes are Organic compounds, produced in the living cells to speed up chemical reaction in the biological systems so that they can take place at relatively lower temperature, but themselves remain apparently unchanged during the process. Therefore enzymes are termed as biocatalysts. Biocatalysts are either proteins (enzymes) or, in a few cases, they may be nucleic acids (ribozymes; some RNA molecules can catalyze the hydrolysis of RNA. Today, we know that enzymes are necessary in all living systems, to catalyze all chemical reactions required for their survival and reproduction – rapidly, selectively and efficiently. Isolated enzymes can also catalyze these reactions. In the case of enzymes however, the question whether they can also act as catalysts outside living systems had been a point of controversy among biochemists in the beginning of the twentieth century. It was shown at an early stage however that enzymes could indeed be used as catalysts outside living cells, and several processes in which they were applied as biocatalysts have been patented These excellent properties of enzymes are utilized in enzyme technology. For example, they can be used as biocatalysts to catalyze chemical reactions on an industrial scale in a sustainable manner. Their application covers the production of desired products for all human material needs (e.g., food, animal feed, pharmaceuticals, fine and bulk chemicals, fibers, hygiene, and environmental technology), as well as in a wide range of analytical purposes, especially in diagnostics. In fact, during the past 50 years the rapid increase in our knowledge of enzymes – as well as their biosynthesis and molecular biology – now allows their rational use as biocatalysts in many processes, and in addition their modification and optimization for new synthetic schemes and the solution of analytical problems

Enzymes have become big business. They are used in many industrial processes to catalyze biological reactions. Enzymes are exploited in a variety of manufacturing processes such as food processing and for the synthesis of medicines such as antibiotics like artificial penicillin. They are also used to clean up factory effluents and pollution in water and soil. Many processes can be made faster and cheaper by using the right enzyme and conditions.

Optimum conditions are maintained during factory production by use of bioreactors. These are vessels which are designed to provide the ideal environment for reactions involving enzymes or living organisms. Source of enzymes used commercial production is plant, animal and microbial cells. Animal enzymes used currently are lipases, tripsin, rennets etc. Most prevalent plant enzymes are papain, proteases, amylases and soybean lipoxygenase. These enzymes are used in food industries, for example, papain extracted from papaya fruit is used as meat tenderizer and pancreatic protease in leather softening and manufacture of detergents. In addition microbial enzymes have gained much popularity. Production of primary and secondary metabolites by microorganism is possible only due to involvement of various enzymes. They are of two types: the extracellular and the intracellular enzymes. There is a wide range of extracellular enzymes produced by pathogenic and saprophytic microorganisms such as cellulose, polymethylegalactouronase, pectinmethylesterase etc. These enzyme helps in establishment in host tissues or decomposition of organic substrates. The intracellular enzyme like invertase, uricoxidase, asparaginase are of high economic value and difficult to extract as they produced inside the cell. They can be extracted by breaking the cells by means of a homogenizer or a ball mill and extracted them through the biochemical process.

Biotechnology offers an increasing potential for the production of goods to meet various human needs. In enzyme technology – a sub-field of biotechnology – new processes have been and are being developed to manufacture both bulk and high added- value products utilizing enzymes as biocatalysts, in order to meet needs such as food (e.g., bread, cheese, beer, vinegar), fine chemicals (e.g., amino acids, vitamins), and pharmaceuticals. Enzymes are also used to provide services, as in washing and environmental processes, or for analytical and diagnostic purposes. The driving force in the development of enzyme technology, both in academia and industry, has been and will continue to be:

  • The development of new and better products, processes and services to meet these needs; and/or

  • The improvement of processes to produce existing products from new raw materials as    biomass.

The goal of these approaches is to innovative products and processes that are not only competitive but also meet criteria of sustainability. A positive effect in all these three fields is required for a sustainable process. Criteria for the quantitative evaluation of the economic and environmental impact are in contrast with the criteria for the social impact, easy to formulate. In order to be economically and environmentally more sustainable than an existing processes, a new process must be designed to reduce not only the consumption of resources (e.g., raw materials, energy, air, water), waste production and environmental impact, but also to increase the recycling of waste per kilogram of product.

Sources of enzymes: Biologically active enzymes may be extracted from any living organism. A very wide range of sources are used for commercial enzyme production from Actinoplanes to Zymomonas, from spinach to snake venom. Of the hundred or so enzymes being used industrially, over a half are from fungi and yeast and over a third are from bacteria with the remainder divided between animal (8%) and plant (4%) sources. A very much larger number of enzymes find use in chemical analysis and clinical diagnosis. Non-microbial sources provide a larger proportion of these, at the present time. Microbes are preferred to plants and animals as sources of enzymes because:

  1. they are generally cheaper to produce.

  2. their enzyme contents are more predictable and controllable,

  3. reliable supplies of raw material of constant composition are more easily arranged, and

  4. plant and animal tissues contain more potentially harmful materials than microbes, including phenolic compounds (from plants), endogenous enzyme inhibitors and proteases.

Table 1 . Some important industrial enzymes and their sources.

Enzyme

EC number

Source

Intra/extra
-cellular

Scale of production

Industrial  use

Animal enzymes

Catalase

1.11.1.6

Liver

I

-

Food

Chymotrypsin

3.4.21.1

Pancreas

E

-

Leather

Lipase

3.1.1.3

Pancreas

E

-

Food

Rennet

3.4.23.4

Abomasum

E

+

Cheese

Trypsin

3.4.21.4

Pancreas

E

-

Leather

Plant enzymes

Actinidin

3.4.22.14

Kiwi fruit

E

-

Food

a-Amylase

3.2.1.1

Malted barley

E

+++

Brewing

b-Amylase

3.2.1.2

Malted barley

E

+++

Brewing

Bromelain

3.4.22.4

Pineapple latex

E

-

Brewing

b-Glucanase

3.2.1.6

Malted barley

E

++

Brewing

Ficin

3.4.22.3

Fig latex

E

-

Food

Lipoxygenase

1.13.11.12

Soybeans

I

-

Food

Papain

3.4.22.2

Pawpaw latex

E

++

Meat

Bacterial enzymes

a-Amylase

3.2.1.1

Bacillus

E

+++

Starch

b-Amylase

3.2.1.2

Bacillus

E

+

Starch

Asparaginase

3.5.1.1

Escherichia coli

I

-

Health

Glucose isomerase

5.3.1.5

Bacillus

I

++

Fructose syrup

Penicillin amidase

3.5.1.11

Bacillus

I

-

Pharmaceutical

Protease

3.4.21.14

Bacillus

E

+++

Detergent

Pullulanase

3.2.1.41

Klebsiella

E

-

Starch

Fungal enzymes

a-Amylase

3.2.1.1

Aspergillus

E

++

Baking

Aminoacylase

3.5.1.14

Aspergillus

I

-

Pharmaceutical

Glucoamylase

3.2.1.3

Aspergillus

E

+++

Starch

Catalase

1.11.1.6

Aspergillus

I

-

Food

Cellulase

3.2.1.4

Trichoderma

E

-

Waste

Dextranase

3.2.1.11

Penicillium

E

-

Food

Glucose oxidase

1.1.3.4

Aspergillus

I

-

Food

Lactase

3.2.1.23

Aspergillus

E

-

Dairy

Lipase

3.1.1.3

Rhizopus

E

-

Food

Rennet

3.4.23.6

Mucor miehei

E

++

Cheese

Pectinase

3.2.1.15

Aspergillus

E

++

Drinks

Pectin lyase

4.2.2.10

Aspergillus

E

-

Drinks

Protease

3.4.23.6

Aspergillus

E

+

Baking

Raffinase

3.2.1.22

Mortierella

I

-

Food

Yeast enzymes

Invertase

3.2.1.26

Saccharomyces

I/E

-

Confectionery

Lactase

3.2.1.23

Kluyveromyces

I/E

-

Dairy

Lipase

3.1.1.3

Candida

E

-

Food

Raffinase

3.2.1.22

Saccharomyces

I

-

Food

Once the enzyme has been purified to the desired extent and concentrated, the manufacturer's main objective is to retain the activity. Enzymes for industrial use are sold on the basis of overall activity. To achieve stability, the manufacturer should follow the recent advanced technology even genetic engineering thechniques.Most industrial enzymes contain relatively little active enzyme (< 10% w/w, including isoenzymes and associated enzyme activities), the rest being due to inactive protein, stabilisers, preservatives, salts and the diluent which allows standardisation between production batches of different specific activities.The key to maintaining enzyme activity is maintenance of conformation, so preventing unfolding, aggregation and changes in the covalent structure. Three approaches are possible: use of additives, the controlled use of covalent modification, and enzyme immobilization. So if the genetic engineering along with the advanced technique for enzyme engineering are employed there might be the great possibility of increasing the half life of active protein and their stability as well as specificity which will certainly reduce conventional methods for stabilizing the enzymes.

Screening for novel enzymes: One of the major skills of enzyme companies and suitably funded academic laboratories is the rapid and cost-effective screening of microbial cultures for enzyme activities. Natural samples, usually soil or compost material found near high concentrations of likely substrates, are used as sources of cultures.

Preparation of enzymes: After the screening of the novel enzyme having great commercial as well as industrial use, enzyme is prepared by optimizing the condition of higher production with available resources. Purification of enzyme after preparation depends upon its future use. Often the enzyme may be purified several hundred-fold but the yield of the enzyme may be very poor, frequently below 10% of the activity of the original material. In contrast, industrial enzymes will be purified as little as possible, only other enzymes and material likely to interfere with the process which the enzyme is to catalyze, will be removed.                         Fig.1 Flow diagram for the preparation of enzymes.

Genetic Protein Engineering of Enzymes


A most exciting development over the last few years is the application of genetic engineering techniques to enzyme technology. Recombinant DNA technology has allowed the transfer of useful enzyme genes from one organism to another. Thus, when an enzyme has been identified as a good candidate enzyme for industrial use, the relevant gene can be cloned into a more suitable production host microorganism and an industrial fermentation carried out. In this way, it becomes possible to produce industrial enzymes of very high quality and purity. A recent example of this technology is the detergent enzyme Lipolase produced by Novo Nordisk A/S, which has improved removal of fat stains in fabrics. The enzyme was first identified in the fungus Humicola languinosa at levels inappropriate for commercial production. The gene DNA fragment for the enzyme was cloned into the fungus Aspergillus oryzae and commercial levels of enzyme achieved. The enzyme has proved to be efficient under many wash conditions. The enzyme is also very stable at a variety of temperature and pH conditions relevant to washing.

There are a number of properties which may be improved or altered by genetic engineering including the yield and kinetics of the enzyme, the ease of downstream processing and various safety aspects. Enzymes from dangerous or unapproved microorganisms and from slow-growing or limited plant or animal tissue may be cloned into safe high-production microorganisms.

All proteins, including enzymes, are based on the same 20 different amino acid building blocks arranged in different sequences. Enzyme proteins typically comprise sequences of several

hundred amino acids folded in a unique three-dimensional structure. Only the sequence of these 20 building blocks determines the three-dimensional structure, which in turn determines all properties such as catalytic activity, specificity and stability. Nature has been performing ‘protein engineering’ for billions of years since the very start of evolution. Natural spontaneous mutations in the DNA coding for a given protein result in changes of the protein structure and hence its properties. This natural variation is part of the adaptive evolutionary process continuously taking place in all living organisms, allowing them to survive in continuously changing environments. Natural variants of enzyme proteins are adapted to perform efficiently in different environments and conditions. This explains why in nature enzymes belonging to the same enzyme family but isolated from different organisms and environments often show a variation in amino acid sequence of more than 50%. The properties of enzymes used for industrial purposes sometimes also require some adaptations in order to function more effectively in applications for which they were not designed by nature. Traditionally, such enzyme optimization is performed by screening naturally occurring microorganisms, followed by classical mutation and selection. The disadvantage of this method is, however, that it may take a very long time until the enzyme with the desired properties is found. This is why protein engineering was developed.

Assumptions for Protein Engineering

While attempting protein engineering, one should recognize the following properties of enzymes:

(i) many amino acid substitutions, deletions or additions lead to no change in enzyme activity, so that they are silent mutations;

(ii) proteins have a limited number of basic structures and only minor changes are superimposed on them leading to variation;

(iii) similar patterns of chain folding and domain structure can arise from different amino acid sequences, which show little or no homology (although same amino acid sequence never gives different folding and domain structures).

The above properties suggest that while many major changes sometimes may lead to no alteration in function, some of the minor changes at specific positions may lead to the desired favourable change.

For example, a single amino acid replacement (glycine to aspartic acid) in E. coli asparate transcarbamylase leads to

(i) loss of activity and to

(ii) an alteration in the binding of catalytic and regulatory subunits. Another example involved the engineering of a single chain biosynthetic antibody binding site (BARS), which is though only one sixth of the size of the complete antibody, but retains its antigen binding specificity.

This synthetic fragment has heavy and light chain variable regions (V H and V J connected by a 15 - amino acid linker. A synthetic gene has also been prepared for the fragment, which expressed in E. coli. This fragment binds to digoxin, a cradiac glycoside. Single amino acid replacements in BABS fragment have sometimes led to major changes in its binding affinity.

In view of the above, it is necessary to examine not only the crystal structure but also the active sites therein, so that the gene may be modified or artificially synthesized for protein engineering to meet the desired needs.

Methods for Protein Engineering

A variety of methods have been used and proposed for future use in protein engineering. In this connection mutagenesis, selection, and recombinant DNA are being used and will be increasingly utilized in future.

1. Mutagenesis and Selection for Protein Engineering - Mutagenesis and selection can be effectively utilized for improving a specific property of an enzyme. Following are some of the examples of selection of mutant enzymes:

(i) E. coli anthranilate synthetase enzyme is normally sensitive to tryptophan inhibition due to feedback inhibition. An MTR 2 mutation of E. coli was found to possess an altered form of enzyme anthranilate synthetase that is insensitive to tryptophan inhibition. They may help in continuous synthesis of tryptophan without any inhibition by tryptophan accumulated as a product.

(ii) Xanthine dehydrogenase enzyme oxidizes 2 hydroxy-purine at position 8, but a mutant has been inolated which oxidizes 2 hydroxy-purine at position 6.

(iii) Lactate dehydrogenase (LDU) from a bacterial system was modified to malate dehydrogenase able a natural mutation leading to a single amino acid substitution (Gln 02... Arg; see later m thIS chapter).

In the above and other cases of naturally occurring mutant enzymes, single amino acid modification or addition/deletion has been observed.

However, if improvement requires changes in several amino acids, such a mutant will be rare or nonexistent and modifications of this type will be possible only through gene modification techniques discussed in the following section.

2. Production of Artificial Semi Synthetic Oxido Reductases - Flavo Enzymes - Artificial oxido reductases can be prepared by covalently attaching redoxactive prosthetic groups to existing sites. Linking of 10-methyilsoalloxazine derivatives (as redox-active groups) to specific sites of several proteins has been achieved. The efficiency of these semisynthetic enzymes (e.g. flavopapain) compares favourably with that of naturally occurring flavoenzymes.

3. Modification of Proteases into Peptide Ligases -Peptide ligation to native enzymes may lead to high specificity and stereoselecitivity, and may suppress side reactions. Therefore, synthesis of any enzyme that may catalyze peptide ligation will be most welcome.

Protease 'subtilisin' has been modified (by converting a serine into cysteine or seleno-cysteine) into thiol-and selenolsubtilisin, the two semi synthetic enzymes (they are damaged proteases), which can catalyse peptide ligation. Both these damaged proteases are efficient peptide ligases. Similarly histidine residue can also be modified to yield peptide ligases.

4. Enzyme PEG Conjugates - An enzyme L- asparaginase (isolated from microbes) has antitumour properties, but is toxic with a life time of less then 18hr thus reducing its utility. It has been shown that E. coli L­-asparaginase can be modified by polyethylene glycol derivatives to produce PEG-asparaginase conjugates , which differ from the native enzyme in following features:
(i) it retains only 52% of the catalytic activity of native enzyme;
(ii) it becomes resistant to proteolytic degradation; (Hi) it does not cause allergy. In view of this, PEG-asparaginase has been used to treat malignant murine (mouse), canine (cats, etc.) and human tumours. PEG conjugates of a large number of enzymes (adenosine deaminase, uricase, catalase, etc.) have been prepared and will be utilized in industry also.

5. Production of Site Specific Nucleases - Restriction Enzymes - The DNA recognition and binding properties of proteins can be combined using chemical cleavage agents. Cys178 of E. coli CAP protein; has been modified using 'S-iodoacetamide -1, 10- phenanthroline' yielding a DNA cleaving agent that recognized and cleaved DNA at the centre of the recognition site (22 bp) for CAP.

This may give restriction enzymes recognizing upto 20 bases instead of 6 or 8 bases and may, therefore, be useful for isolating long DNA fragments needed for sequencing and mapping. Nucleases may also be produced by fusion of non-specific phosphodiesterases to oligonucleotides of defined sequence.

For a nuclease from Staphylococcus modified by this approach, it was shown that oligonucleotide component of fused product pairs with its complementary sequence and the hybrid enzyme hydrolyses single stranded DNA or RNA adjacent to the oligonucleotide binding site. This approach thus can also be used for developing artificial restriction enzymes.

Protein engineering and how it is applied to enzymes

A most exciting development over the last few years is the application genetic engineering techniques to enzyme technology. Protein engineering of enzymes is a faster, more controlled, more targeted and more accurate method to optimize the properties of enzymes for a specific industrial application than the traditional method described above. It makes it possible to sidestep the high number of natural isolate screenings that would otherwise be necessary to find the enzyme with the desired properties, and increases the likelihood that a suitable enzyme will be found. The protein engineering technique involves genetic modification by means of recombinant DNA technology of the enzyme producing microorganism, in particular the enzyme encoding gene, resulting in substitution of one or more amino acids in the amino acid sequence of the enzyme protein. Strategies for making such amino acid substitutions and developing protein engineered enzymes are based on the knowledge of the structure/function relationships of enzymes, computer modeling and techniques for creating and testing enzyme variants.

Enzyme technology is the application of modifying an enzyme's structure (and thus its function) or modifying the catalytic activity of isolated enzymes to produce new metabolites, to allow new (catalyzed) pathways for reactions to occur, or to convert from some certain compounds into others (biotransformation). These products will be useful as chemicals, pharmaceuticals, fuel, food or agricultural additives. An enzyme reactor consists of a vessel containing a reactional medium that is used to perform a desired conversion by enzymatic means. Enzymes used in this process are free in the solution or immobilized in particulate, membranous or fibrous support. There are many directions in which enzyme technologists are currently applying their art and which are at the forefront of biotechnological research and development. Some of these have already been examined in some detail earlier. At present, relatively few enzymes are available on a large scale (i.e. > kg) and are suitable for industrial applications. These shortcomings are being addressed in a number of ways:

  1. New enzymes are being sought in the natural environment and by strain selection

  2. Novel enzymes are being designed and produce by genetic engineering;

  3. New organic catalysts are being designed and synthesized using the 'knowhow' established from enzymology; and

  4. More complex enzyme systems are being utilized.

Each of these areas has a extensive and rapidly expanding literature. Some advances possibly belong more properly to other areas of science. Thus, the development of genetically improved enzymes is generally undertaken by molecular biologists and the and synthesis of novel enzyme-like catalysts is in the provenance of the organic chemists. Both groups of workers will, however, base their science on data provided by the enzyme technologist.

There are a number of properties which may be improved or altered by genetic engineering including the yield and kinetics of the enzyme, the ease of downstream processing and various safety aspects. Enzymes from dangerous or unapproved microorganisms and from slow growing or limited plant or animal tissue may be cloned into safe high-production microorganisms. In the future, enzymes may be redesigned to fit more appropriately into industrial processes; for example, making glucose isomerase less susceptible to inhibition by the Ca2+ present in the starch saccharification processing stream.

The amount of enzyme produced by a microorganism may be increased by increasing the number of gene copies that code for it. This principle has been used to increase the activity of penicillin-G-amidase in Escherichia coli. The cellular DNA from a producing strain is selectively cleaved by the restriction endonuclease HindIII. This hydrolyses the DNA at relatively rare sites containing the 5'-AAGCTT-3' base sequence to give identical 'staggered' ends.

[Fig2]
intact DNA cleaved DNA

The total DNA is cleaved into about 10000 fragments, only one of which contains the required genetic information. These fragments are individual cloned into a cosmid vector and thereby returned to E. coli. These colonies containing the active gene are identified by their inhibition of a 6-amino-penicillanic acid-sensitive organism. Such colonies are isolated and the penicillin-G-amidase gene transferred on to pBR322 plasmids and recloned back into E. coli. The engineered cells, aided by the plasmid amplification at around 50 copies per cell, produce penicillin-G-amidase constitutively and in considerably higher quantities than does the fully induced parental strain. Such increased yields are economically relevant not just for the increased volumetric productivity but also because of reduced downstream processing costs, the resulting crude enzyme being that much purer.

The process starts with the isolation and characterisation of the required enzyme. This information is analysed together with the database of known and putative structural effects of amino acid substitutions to produce a possible improved structure. This factitious enzyme is constructed by site-directed mutagenesis, isolated and characterised. The results, successful or unsuccessful, are added to the database, and the process repeated until the required result is obtained.

Another extremely promising area of genetic engineering is protein engineering. New enzyme structures may be designed and produced in order to improve on existing enzymes or create new activities. An outline of the process of protein engineering is shown in Figure 2. Such factitious enzymes are produced by site-directed mutagenesis (Figure 3). Unfortunately from a practical point of view, much of the research effort in protein engineering has gone into studies concerning the structure and activity of enzymes chosen for their theoretical importance or ease of preparation rather than industrial relevance. This emphasis is likely to change in the future. Figure 2. The protein engineering cycle.

As indicated by the method used for site-directed mutagenesis (Figure 3), the preferred pathway for creating new enzymes is by the stepwise substitution of only one or two amino acid residues out of the total protein structure. Although a large database of sequence-structure correlations is available, and growing rapidly together with the necessary software, it is presently insufficient accurately to predict three-dimensional changes as a result of such substitutions. The main problem is assessing the long-range effects, including solvent interactions, on the new structure. As the many reported results would attest, the science is at a stage where it can explain the structural consequences of amino acid substitutions after they have been determined but cannot accurately predict them. Protein engineering, therefore, is presently rather a hit or miss process which may be used with only little realistic likelihood of immediate success. Apparently quite small sequence changes may give rise to large conformational alterations and even affect the rate-determining step in the enzymic catalysis. However it is reasonable to suppose that, given a sufficiently detailed database plus suitable software, the relative probability of success will increase over the coming years and the products of protein engineering will make a major impact on enzyme technology.

Much protein engineering has been directed at subtilisin (from Bacillus amyloliquefaciens), the principal enzyme in the detergent enzyme preparation, Alcalase. This has been aimed at the improvement of its activity in detergents by stabilising it at even higher temperatures, pH and oxidant strength. Most of the attempted improvements have concerned alterations to:

  1. the P1 cleft, which holds the amino acid on the carbonyl side of the targeted peptide bond;

  2. the oxyanion hole (principally Asn155), which stabilises the tetrahedral intermediate;

  3. the neighbourhood of the catalytic histidyl residue (His64), which has a general base role; and

  4. the methionine residue (Met222) which causes subtilisin's lability to oxidation.

It has been found that the effect of a substitution in the P1 cleft on the relative specific activity between substrates may be fairly accurately predicted even though predictions of the absolute effects of such changes are less successful. Many substitutions, particularly for the glycine residue at the bottom of the P1 cleft (Gly166), have been found to increase the specificity of the enzyme for particular peptide links whilst reducing it for others. These effects are achieved mainly by corresponding changes in the Km rather than the Vmax. Increases in relative specificity may be useful for some applications. They should not be thought of as the usual result of engineering enzymes, however, as native subtilisin is unusual in being fairly non-specific in its actions, possessing a large hydrophobic binding site which may be made more specific relatively easily (e.g. by reducing its size). The inactivation of subtilisin in bleaching solutions coincides with the conversion of Met222 to its sulfoxide, the consequential increase in volume occluding the oxyanion hole. Substitution of this methionine by serine or alanine produces mutants that are relatively stable, although possessing somewhat reduced activity.

Figure 3. An outline of the process of site-directed mutagenesis, using a hypothetical example. (a) The primary structure of the enzyme is derived from the DNA sequence. A putative enzyme primary structure is proposed with an asparagine residue replacing the serine present in the native enzyme. A short piece of DNA (the primer), complementary to a section of the gene apart from the base mismatch, is synthesised. (b) The oligonucleotide primer is annealed to a single-stranded copy of the gene and is extended with enzymes and nucleotide triphosphates to give a double-stranded gene. On reproduction, the gene gives rise to both mutant and wild-type clones. The mutant DNA may be identified by hybridisation with radioactively labelled oligonucleotides of complementary structure.

An example of the unpredictable nature of protein engineering is given by trypsin, which has an active site closely related to that of subtilisin. Substitution of the negatively charged aspartic acid residue at the bottom of its P1 cleft (Asp189), which is used for binding the basic side-chains of lysine or arginine, by positively charged lysine gives the predictable result of abolishing the activity against its normal substrates but unpredictably also gives no activity against substrates where these basic residues are replaced by aspartic acid or glutamic acid.

Considerable effort has been spent on engineering more thermophilic enzymes. It has been found that thermophilic enzymes are generally only 20-30 kJ more stable than their mesophilic counterparts. This may be achieved by the addition of just a few extra hydrogen bonds, an internal salt link or extra internal hydrophobic residues, giving a slightly more hydrophobic core. All of these changes are small enough to be achieved by protein engineering. To ensure a more predictable outcome, the secondary structure of the enzyme must be conserved and this generally restricts changes in the exterior surface of the enzyme. Suitable for exterior substitutions for increasing thermostability have been found to be aspartate , glutamate, lysine , glutamine, valine , threonine, serine , asparagine, isoleucine , threonine, asparagine , aspartate and lysine , arginine. Such substitutions have a fair probability of success. Where allowable, small increases in the interior hydrophobicity for example by substituting interior glycine or serine residues by alanine may also increase the thermostability. It should be recognised that making an enzyme more thermostable reduces its overall flexibility and, hence, it is probable that the factitious enzyme produced will have reduced catalytic efficiency.

Artificial enzymes:

A number of possibilities now exist for the construction of artificial enzymes. These are generally synthetic polymers or oligomers with enzyme-like activities, often called synzymes. They must possess two structural entities, a substrate-binding site and a catalytically effective site. It has been found that producing the facility for substrate binding is relatively straightforward but catalytic sites are somewhat more difficult. Both sites may be designed separately but it appears that, if the synzyme has a binding site for the reaction transition state, this often achieves both functions. Synzymes generally obey the saturation Michaelis-Menten kinetics . For a one-substrate reaction the reaction sequence is given by

synzyme + S (synzyme-S complex) synzyme + P

Some synzymes are simply derivatised proteins, although covalently immobilised enzymes are not considered here. An example is the derivatisation of myoglobin, the oxygen carrier in muscle, by attaching (Ru(NH3)5)3+ to three surface histidine residues. This converts it from an oxygen carrier to an oxidase, oxidising ascorbic acid whilst reducing molecular oxygen. The synzyme is almost as effective as natural ascorbate oxidases.

It is impossible to protein synzymes from scratch with any probability of success, as their conformations are not presently predictable from their primary structure. Such proteins will also show the drawbacks of natural enzymes, being sensitive to denaturation, oxidation and hydrolysis. For example, polylysine binds anionic dyes but only 10% as strongly as the natural binding protein, serum albumin, in spite of the many charges and apolar side-chains. Polyglutamic acid, however, shows synzymic properties. It acts as an esterase in much the same fashion as the acid proteases, showing a bell-shaped pH-activity relationship, with optimum activity at about pH 5.3, and Michaelis-Menten kinetics with a Km of 2 mm and Vmax of 10-4 to 10-5 s-1 for the hydrolysis of 4-nitrophenyl acetate. Cyclodextrins (Schardinger dextrins) are naturally occurring toroidal molecules consisting of six, seven, eight, nine or ten a-1, 4-linked D-glucose units joined head-to-tail in a ring (a-, b-, g-, d- and e-cyclodextrins, respectively: they may be synthesised from starch by the cyclomaltodextrin glucanotransferase (EC 2.4.1.19) from Bacillus macerans). They differ in the diameter of their cavities (about 0.5-1 nm) but all are about 0.7 nm deep. These form hydrophobic pockets due to the glycosidic oxygen atoms and  inwards-facing C-H groups. All the C-6 hydroxyl groups project to one end and all the C-2 and C-3 hydroxyl groups to the other. Their overall characteristic is hydrophilic, being water soluble, but the presence of their hydrophobic pocket enables them to bind hydrophobic molecules of the appropriate size. Synzymic cyclodextrins are usually derivatised in order to introduce catalytically relevant groups. Many such derivatives have been examined. For example, a C-6 hydroxyl group of b-cyclodextrin was covalently derivatised by an activated pyridoxal coenzyme. The resulting synzyme not only acted a transaminase but also showed stereoselectivity for the L-amino acids. It was not as active as natural transaminases, however. Polyethyleneimine is formed by polymerising ethyleneimine to give a highly branched hydrophilic three-dimensional matrix. About 25% of the resultant amines are primary, 50% secondary and 25% tertiary:Ethyleneimine                      polyethyleneimine

The primary amines may be alkylated to form a number of derivatives. If 40% of them are alkylated with 1-iodododecane to give hydrophobic binding sites and the remainder alkylated with 4(5)-chloromethylimidazole to give general acid-base catalytic sites, the resultant synzyme has 27% of the activity of a-chymotrypsin against 4-nitrophenyl esters. As might be expected from its apparently random structure, it has very low esterase specificity. Other synzymes may be created in a similar manner.

Antibodies to transition state analogues of the required reaction may act as synzymes. For example, phosphonate esters of general formula (R-PO2-OR')- are stable analogues of the transition state occurring in carboxylic ester hydrolysis. Monoclonal antibodies raised to immunising protein conjugates covalently attached to these phosphonate esters act as esterases. The specificities of these catalytic antibodies (also called abzymes) depends on the structure of the side-chains (i.e. R and R' in (R-PO2-OR')-) of the antigens. The Km values may be quite low, often in the micromolar region, whereas the Vmax values are low (below 1 s-1), although still 1000-fold higher than hydrolysis by background hydroxyl ions. A similar strategy may be used to produce synzymes by molecular 'imprinting' of polymers, using the presence of transition state analogues to shape polymerising resins or inactive non-enzymic protein during heat denaturation.

Coenzyme-regenerating systems

Many oxidoreductases and all ligases utilise coenzymes (e.g. NAD+, NADP+, NADH, NADPH, ATP), which must be regenerated as each product molecule is formed. Although these represent many of the most useful biological catalysts, their application is presently severely limited by the high cost of the coenzymes and difficulties with their regeneration. These two problems may both be overcome at the same time if the coenzyme is immobilised, together with the enzyme, and regenerated in situ.

A simple way of immobilising/regenerating coenzymes would be to use whole-cell systems and these are, of course, in widespread use. However as outlined earlier, these are of generally lower efficiency and flexibility than immobilised-enzyme systems. Membrane reactors (may be used to immobilise the coenzymes but the pore size must be smaller than the coenzyme diameter, which is extremely restrictive. Coenzymes usually must be derivatised for adequate immobilisation and regeneration. When successfully applied, this process activates the coenzymes for attachment to the immobilisation support but does not interfere with its biological function. The most widely applied synthetic routes involve the alkylation of the exocyclic N6-amino nitrogen of the adenine moiety present in the coenzymes NAD+, NADP+, NADH, NADPH, ATP and coenzyme A.

In some applications, such as those using membrane reactors it is only necessary that the coenzyme has sufficient size to be retained within the system. High molecular weight water-soluble derivatives are most useful as they cause less diffusional resistance than insoluble coenzyme matrices. Dextrans, polyethyleneimine and polyethylene glycols are widely used. Relatively low levels of coenzyme attachment are generally sought in order to allow greater freedom of movement and avoid possible inhibitory effects. The kinetic properties of the derived coenzymes vary, depending upon the system, but generally the Michaelis constants are higher and the maximum velocities are lower than with the native coenzymes. Coenzymes immobilised to insoluble supports presently have somewhat less favourable kinetics even when co-immobilised close to the active site of their utilising enzymes. This situation is expected to improve as more information on the protein conformation surrounding the enzymes' active sites becomes available and immobilisation methods become more sophisticated. However, the cost of such derivatives is always likely to remain high and they will only be economically viable for the production of very high value products.

There are several systems available for the regeneration of the derivatised coenzymes by chemical, electrochemical or enzymic means. Enzymic regeneration is advantageous because of its high specificity but electrochemical procedures for regenerating the oxidoreductase dinucleotides are proving competitive. To be useful in regenerating coenzymes, enzymic processes must utilise cheap substrates and readily available enzymes and give non-interfering and easily separated products. Formate dehydrogenase and acetate kinase present useful examples of their use, although the presently available commercial enzyme preparations are of low activity:

Genetically Engineered Enzymes

Enzymes are naturally occurring proteins that speed up biochemical processes. They're used to produce everything from wine and cheese to corn syrup and baked goods. Enzymes allow the manufacturer to produce more of a particular product in a shorter amount of time, thus increasing profit.

Generally, the use of enzymes is beneficial. In some cases, they can replace harmful chemicals and reduce water and energy consumption in food production. However, enzymes produced by genetically engineered organisms are cause for concern. Not enough is known about the long-term effects of these enzymes on humans and the ecosystem for them to be used across the board.

FDA regulations on enzyme use is a gray area. Enzymes used in the processing of foods do not have to be listed on product labels because they are not considered foods. Also, when enzymes are genetically engineered, the manufacturer is not required to notify the FDA that the enzymes have been modified. The lists of GE enzymes known by the FDA is, by their own admission, "probably incomplete."

Worldwide, the enzyme market is a $1.3 billion industry. One of the largest enzyme manufacturers are Novo Nordisk, which manufactures GE and non-GE enzymes. The FDA provided us with this partial list of genetically engineered enzymes:

  • Chymosin—used in the production of cheese

  • Novamyl(TM)—used in baked goods to help preserve freshness

  • Alpha amylase—used in the production of white sugar, maltodextrins and nutritive carbohydrate           sweeteners  (corn syrup)

  • Aspartic (proteinase enzyme from R. miehei)—used in the production of cheese

  • Pullulanase—used in the production of high fructose corn syrup

If you want to absolutely avoid genetically engineered enzymes you will have two choices: avoid foods in the following categories, or call the food manufacturers directly and ask them if their enzymes are genetically engineered. They will probably have no idea. Ask them to check and call them back again. Let us know if you get written confirmation.

  • Beers, wines and fruit juices—(Enzymes used: Cereflo, Ceremix, Neutrase, Ultraflo, Termamyl, Fungamyl, AMG, Promozyme, Viscozyme, Finizym, Maturex, Pectinex, Pectinex Ultra SP-L, Pectinex BE-3L, Pectinex AR, Ultrazym, Vinozym, Citrozym, Novoclairzym, Movoferm 12, Glucanex, Bio-Cip Membrane, Peelzym, Olivex/Zietex)

  • Sugar—Enzymes used: Termamyl, Dextranase, Invertase, Alpha Amylase

  • Oils—Enzymes used: Lipozyme IM, Novozym 435, Lecitase, Lipozyme, Novozym 398, Olivex, Zeitex

  • Dairy products—Enzymes used: Lactozym, Palatase, Alcalase, Pancreatic Trypsin Novo (PTN), Flavourzyme, Catazyme, Chymosin

  • Baked goods—Enzymes used: Fungamyl, AMG, Pentopan, Novomyl, Glutenase, Gluzyme

In many cases the enzymes named above are brand names. They may appear under other names as well. Enzymes are usually found in minuscule quantities in the final food product. The toxin found in genetically engineered tryptophan was less than 0.1 percent of the total weight of the product, yet it was enough to kill people. The use of enzymes is pervasive in the food industry. Nothing is known about the long-term effects of genetically engineered enzymes. We include this information so you can make an informed choice about whether you want to eat them or not.

Enzymes produced by genetically modified microorganisms

Novozymes’ enzymes produced by genetically modified microorganisms

Novozymes A/S markets a range of enzymes for various industrial purposes. Many of these enzymes are produced by fermentation of genetically modified microorganisms (GMMs).

There are several advantages of using GMMs for the production of enzymes, including:

  • It is possible to produce enzymes with a higher specificity and purity

  • It is possible to obtain enzymes which would otherwise not be available for economical, occupational health or environmental reasons

  • Due to higher production efficiency there is an additional environmental benefit through reducing energy consumption and waste from the production plants

  • For enzymes used in the food industry particular benefits are for example a better use of raw materials (juice industry), better keeping quality of a final food and thereby less wastage of food (baking industry) and a reduced use of chemicals in the production process (starch industry)

  • For enzymes used in the feed industry particular benefits include a significant reduction in the amount of phosphorus released to the environment from farming

Due to an efficient separation process the final enzyme product does not contain any GMMs.

The enzymes are produced by fermentation of the genetically modified micro organisms (the production strain) which then produces the desired enzyme. The process takes place under well-controlled conditions in closed fermentation tank installations.

After fermentation the enzyme is separated from the production strain, purified and mixed with inert diluents for stabilisation.

The following is a list of Novozymes' enzymes produced by genetically modified organisms.

Food Applications:

Brand name

Type of enzymes

Main Application

Amylase® AG XXL

Glucoamylase

Juice Industry

Dextrozyme®

Pullulanase / Amyloglucosidase

Starch industry

Finizym® W

Phospholipase

Starch industry

Gluzyme® Mono

Glucose oxidase

Baking industry

Lecitase® Novo

Lipase

Oils and fats industry

Maltogenase®

Maltogenic amylase

Starch industry

Maturex®

Alpha-acetodecarboxylase

Brewing industry

NovoCarne® Tender

Protease

Meat industry

Novoshape®

Pectinesterase

Fruit processing

Novozym® 27080

Carbohydrase / Lipase

Baking industry

NOVOZYM® 27122

Xylanase

Protein Hydrolysis

Novozym® 33081

Polygalacturonase

Juice Industry

Novozym® 46016

Phospholipase

Dairy industry

Novozym® 46019

Cellobiose oxidase

Dairy Industry

Pectinex® XXL

Pectin lyase / Polygalacturonase

Juice Industry

Promozyme® D2

Pullulanase

Starch industry

Saczyme®

Glucoamylase

Alcohol Industry

Toruzyme®

Transferase

Starch industry

Feed Applications:

Brand name

Type of enzymes

Main Application

Bio-Feed® Wheat

Xylanase

Animal feed industry

Bio-feed® Phytase

Phytase

Animal feed industry

Other Applications:

Brand name

Type of enzymes

Main Application

Alcalase®

Subtillisin

Detergent industry

Aquazym® LT-L

Alpha-amylase

Textile industry

BioPrep®

Pectate lyase

Textile industry

Carezyme®

Cellulase

Detergent industry

Clear-Lens® LIPO

Lipase

Personal care industry

DeniLite®

Laccase

Textile industry

DeniMax® 601

Cellulase

Textile Industry

Duramyl®

Alpha-amylase

Detergent industry

Everlase®

Subtillisin

Detergent industry

Extruzyme® Pro

Alpha-amylase

Pet food industry

Greasex®

Lipase

Leather industry

Kannase®

Subtillisin

Detergent industry

Lipex®

Lipase

Detergent industry

Lipolase®

Lipase

Detergent industry

Liquanase®

Subtilisin

Detergent industry

Liquozyme®

Alpha-amylase

Starch and Ethanol industry

Mannaway®

Mannanase

Detergent industry

NovoBate® 100

Trypsin

Leather Industry

Chemical Modification of Enzymes

We know that the proteins synthesized under the control of gene sequences in a cell undergo post translational modification. This leads to stability, structural integrity, altered solubility and viscosity of individual proteins. This may also alter the chemical reactivity.

These alterations can be achieved in vitro and may .sometimes even create entirely new enzyme, by creating new active sites or modifying the old ones. Some of the examples will be described in this section.

Protein Modelling

Utilizing the data generated through X-ray diffraction and NMR studies, models can be constructed with the help of computer graphics. There are computer programmes available (interactive colour graphics programmes) with the help of which a protein structure can be fitted to the electron density map (obtained from X-ray diffraction) by simultaneous display on the screen of computer monitor. Similarly, Van der Waals surfaces for the protein can be displayed and interaction between several molecules simulated.

There are also other interactive molecular graphics which can be used (with the help of programmes) to find out the perturbations (disturbances) in protein structure that will result from specific modifications of amino acid sequences. We know that to some extent the three dimensional structure of a protein can be predicted from the amino acid sequence, but we still have to depend partly on X-ray diffraction patterns for determining the three dimensional structure.

In future when the three dimensional structure can be accurately predicted from amino acid sequence data, this will lead to long term success in protein engineering. The models of proteins, made on the basis of amino acid alterations, can then be tested for the predictions about structure function relationships.

Multienzyme Systems by Gene Fusion ( Bi and Polyfunctional Enzymes)

Multienzyme systems have been artificially synthesized, which can catalyze sequential reactions in many biotechnological production processes. Although, proximity of more than one enzymes can also be achieved by co-immobilization and chemical cross linking, gene fusion appears to have the highest potential in enzyme technology. The gene fusion technology, for preparation of bi-and polyfunctional enzymes, involves joining of structural genes of two or more enzymes. The translational stop singal at the 3' end of the first gene is removed and ligated in frame to the A TG start codon of the second gene. Alternatively, short linkers (2-10 amino acids) are used. The novel chimaeric gene gives a single polypeptide chain carrying active sites of both genes. This fusion may involve

(i)     two monomeric enzymes

(ii)   a monomeric and a dimeric enzyme or

(iii) two dimeric enzymes.

Rationale of Protein Enzyme Engineering - Although thousands of proteins have been characterized in prokaryotes and eukaryotes, only few became commercially important. This is due to the high cost of isolating and purifying enzymes in sufficient quantities.

Although the cost aspect has been overcome by producing an enzyme in large quantities in bacteria, for its industrial application, an enzyme (outside the cell) should also have some characteristics in addition to those of enzymes in the cells. These characteristics may include the following:
(i) enzyme should be robust with a long life;

(ii) enzyme should be able to use the substrate supplied in the industry even if it differs slightly from that in the cell;
(iii) enzyme should be able to work under conditions (e.g. extremes of pH, temperature and concentration) of the industry even if they differ from those in the cell.

In view of the above, enzyme should be engineered to meet the altered needs. Therefore, efforts have been made to alter the properties of the enzymes. Following is the list of properties that one needs to alter in a predictable manner for protein or enzyme engineering.

(1)      Kinetic properties of enzyme turnover and Michaelis Constant, Km.
(2) Theremostability and the optimum temperature for the enzyme.
(3) Stability and activity of enzyme in nonaqueous solvents.
(4) Substrate and reaction specificity.
(5) Cofactor requirements.
(6) Optimun pH.
(7) Protease resistance.
(8) Allosteric regulation.
(9) Molecular weight and subunit structure.

For a particular class of enzymes, variation in nature may occur for each of the above properties, so that one may like to combine the optimum properties to get the most efficient form of the enzyme.

This aspect of protein engineering will be illustrated using the example of glucose isomerases, which convert glucose into other isomers like fructose and are used to make high fructose corn syrup vital for soft drink industry. It exhibits wide variation in its properties.
Sometimes, it may not be possible to get a combination of optimum properties. For instance, an enzyme with highest activity may not be the most stable. Therefore, a compromise in properties may have to be made, if we have to select an enzyme from the available variability or even if we create variability by mutagenesis.
However, if structure and function relationship of an enzyme is known, the structural features for desirable function may be combined and protein engineering techniques may then be used to create a novel enzyme exhibiting a combination of all desirable functional properties.

Glucose isomerase belongs to a TIM barrel family of enzymes which resemble each other in having a highly characteristic domain called TIM barrel, with active site for catalytic action at one end. This TIM barrel may be found in enzymes that may differ in sequences and may catalyze different reactions.
As earlier discussed, since similarities of structure of protein meant similarities in function, TIM barrel presents a challenge to this concept. However, it is curious tbat some enzymes in this family appear in pairs in their metabolic pathways so that they catalyse two consecutive steps thus showing coupling of their functions.
As an example of two enzymes of TIM barrel family, while 'triose phosphate isomerase' is one of the most efficient catalysts, 'glucose isomerase' is relatively very inefficient.
Therefore, if 'glucose isomerase' enzyme is redesigned to use the highly efficient domain of TIM barrel family, it will be a remarkable achievement for soft drink industry. Efforts in this direction are being made (see later for methods of protein engineering).

Acheivements of Protein Engineering

A number of proteins are known, now, where efforts have been made to know the effects of site specific mutagenesis involving substitution of one or more amino acids. Efforts have also been made to study in detail the function of different regions of a protein. Following are some results of such efforts.

?-lactamase. This enzyme functions in the periplasmic space of bacterial cells. The enzyme hydrolyses and inactivates the beta- lactam ring of penicillin derivatives and helps in transport across the inner membrane. During transport a polypeptide (signal sequence peptide of 23 amino acids) is cleaved off.

Detailed analysis suggested that, transport and processing does not depend on this polypeptide of 23 amino acids alone. An active site involving amino acid serine has also been identified, since its replacement by cysteine leads to reduction in the activity of this enzyme.

Dihydrofolate reductase. In this enzyme, replacement of a single amino acid, aspartic add (ASP) by asparagine (ASN), led to a decrease in specific activity by a thousand fold, suggesting that aspartic acid is very important.(or the active site. Other similar modifications were also examined.

Insulin. It consists of A and B chains linked by C-peptide of 35 amino acids. It was shown that a sequence of 6 amino acids for C-peptide was adequate for the, linking function.

Lactose permease (product of, gene of 'lac' operon). This enzyme is involved in transport of lactose and a cysteine to glycine substitution showed that this amino acid was not essential for transport. Further, out of four histidine residues, two at positious 35 and '39 do' not play any essential role in transport, while the mutation in any of the other two histidines at positions 208 and 322, lead to loss of transport function.

T4 lysozyme. A mutation of isoleucine to cystine in this enzyme leading to formation of a disulphide bridge led to thermal stability and a 200 fold increase in enzyme activity even at 6T'C.

Human beta interferon. Removal of one of the three cysteine residues' I led to an improvement in stability of the enzyme.

? repressor. This protein could be engineered to develop a specific site for cro protein, since the alteration led to development of a cro recognition site.I

Acetylcholine receptor. This protein is involved in transport, of acetylcholine through. the membrane. Specific regions of this protein involved in acetylcholine binding and channel formation have been, identified.

Cytochrome C. A phenylalanine residue has been identified to be non-essential for electron transfer but is involved in determining the reduction potential of the protein.

Trypsin. It could be redesigned to have altered substrate specificity.

Subtilisin. Another successful alteration of substrate specificity involved the enzyme subtilisin reported in 1986-87.

Lactate dehydrogenase. A lactate dehydrogenase (LDH) from Bacillus stearothermophilus was modified separately by each of the three substitutiens of amino acids (resulting from mutations; Asp197... Asn; Thr246"'Gly; Gln102...Arg). The substitution, Gln102"'Arg, led to change in specificity from lactate to malate, with high efficiency, comparable to that which the native LDH had for lactate.

Lactic protease. Substrate specificity of lactic protease (in E. coli), has been shown to be dramatically modified by replacing active site methionine by alanine (Met19

About the Author

http://sites.google.com/site/micromegabtech/

High Side

 

High Side

High Side
Where is the High side AC service valve on a 1996 Mustang GT?

I know where the low side is. its on the accumulator. I need to know where the other one is, and i can find anything online. Facts only please

No license or certification is required to work on a 96 mustangs ac system it contains R134a witch is better for the environment it contains no floral carbons (cfc's).

Now back to your question the high side service port is located on the discharge hose between the compressor & the ac condensor.

 
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High Blood Pressure - kitchen help You

High Blood Pressure

Today, life has become so stressful that there is hardly any man who is not suffering any kind of disease. Long working hours, unhealthy food habit, insufficient rest and sleep, tension and stress, all leads to different health problems. High blood pressure is one such problem in which the blood pressure rises more than the normal pressure level of 120/80 mm of Hg. This not only is an alarming condition, but it leads to several other heart-related disease, poor functioning of the sense organ, etc. This article will explain, in detail, every aspect of high blood pressure.

  1. Causes for High Blood Pressure
  2. High Blood Pressure Symptoms
  3. Home Remedies for High Blood Pressure

High Blood Pressure Causes

As mentioned above excess stress, unhealthy food habit (especially high calories food, excess intake of salt) all lead to high blood pressure. The other major causes for high blood pressure is alcohol, smoking, excess consumption of tea and coffee, pain killers and other strong medicines, genetic disorder, overweight, problem in thyroid and kidney, irregular heart beat and chest pain, and diabetes

High Blood Pressure Symptoms

Person suffering from high blood pressure suffer lots of problem. It is a kind of silent killer which slowly starts affecting the entire body system. The main high blood pressure symptoms are severe body pain (especially in the neck and the lower part of the head), nervousness, chest pain, high sleeping tendency, weakness, heavy bleeding from nose, inability to control emotions. There are several home remedies for the treatment of high blood pressure. However, the best way to stay away from this disease is not to take too much stress, eating balanced diet, and live a stress-free life.

Home Remedies for High Blood Pressure

High blood pressure is a root cause of several other diseases and has to be cured immediately. With heavy medicines being one cause for this disease, home remedies are highly recommended for its treatment. Given below are some of the helpful and fast relief home remedies for high blood pressure.

Madhu (Honey): Honey is one of the most common home remedy for the treatment of different health-related problems. Take equal amount of honey, ginger juice, and finely powdered cumin (jeera) seeds, approx 2-3 tablespoon, and make a mixture. Take this mixture 2-3 tablespoon twice a day. This is one of the useful home remedies for high blood pressure.

Boiled rice and potato: It is said that patient suffering from high blood pressure should take boiled rice, especially brown rice, in their diet. It regulates and soothes the nerves and thus help in lowering high blood pressure. Brown rice is also rich in minerals like calcium, etc. Similarly, boiled potato is also good. Patient with high blood pressure should take less salt in their diet, and taking potato may carve from excess salt intake.

Gooseberry (amla): Gooseberry or amla too has a positive effect in the treatment of high blood pressure. Take 1-2 tablespoon of amla juice with honey in empty stomach early in the morning.

Onion juice: Take onion juice (2-3 tablespoon) and mix honey (2-3 tablespoon) to it. Take this mixture for the treatment of high blood pressure.

Fenugreek (methi) seeds: Take 1-2 tablespoon of methi seeds and boil in a glass of water. Strain and then take this mixture. This is one of the best home remedy for the treatment of high blood pressure. Patient may continue this drink for 2-3 months twice a day. This is one of the best home remedies for high blood pressure.

Curry leaves: Curry leaves have strong medicinal effect for the treatment of high blood pressure. Take 35-40 green curry leaves and boil in a glass of water. Keep it aside and allow it to cool. Drink it in empty stomach in early morning. Another way of taking curry leaf tea is with two-three tablespoon of lemon extract.

Lemon: Lemon extract also is effective for the treatment of high blood pressure. Take 2-3 tablespoon of lime extract in a cup of water. Freshly prepared lemon juice too has a great effect. This is one of the important home remedies for high blood pressure.

Khus khus (cus-cus grass): Take equal amount of khus khus and chor magaz (150 gm) and grind into fine powder. Take 1-2 tablespoon of this powder with water twice a day. Patient may take the first dose in an empty stomach.

Lahsun (Garlic): Two-three seeds of garlic are the best home remedy for high blood pressure. It has a magical effect in lowering the blood pressure level; it also regulates the heart beat, helps in the proper functioning of the lungs and other parts of the body. It makes the body active and reduces body pain.

Fruits: Various fruits like grapes, water melon, and papaya play vital role in the treatment of high blood pressure. This regulates blood pressure and bring heart beat to normal. The seeds of water melon can also be dried and finely powdered. This powder can be taken 1-2 tablespoon in a glass of water. Take raw papaya in an empty stomach in the early morning. This clears the bowel movement, prevents constipation, and thus reduces high blood pressure.

Vegetables: Vegetables like carrot and spinach too will help in reducing high blood pressure. Both these vegetables and other green leafy vegetables are very helpful. Extract fresh juice from carrot and spinach and take a glass of it twice a day.

First of all a well balanced diet, rich in green vegetables and fruits is a must. The food should be rich in minerals like calcium, etc. Second thing patient should strictly avoid junk foods and do exercise and yoga regularly. Different breathing-related yogas help in reducing body weight, regulating heart beat and thus controlling high blood pressure . Patient should take proper rest at least 6-7 hours sleep daily. Other things to lower the high blood pressure are quitting alcohol and smoking.

About the Author

B.Sc.(Med.), B.Ed., M.A.(Edu.), M.Litt.(Edu.), Ph.D.(Edu.Psy.)PGDCA.

Served as Science Master, Employment Department as Vocational Guidance Officer.

Retired from Employment Department, Punjab India as Dy. Director (Off.)

Serving now Arihant Computer Center and Many Medical Hospitals such as Sadbhavna Medical & Heart Institute.