QBM CH 9

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Bovine serum albumin weight

67kDa

Where is the protein of interest on an SDS PAGE?

Consistant, last protein eluted

Can proteins bind differently to SDS?

It is rare but some do bind SDS differently

Sample loading buffer is also known as

Laemmli Buffer

Advantages of TCE?

Quick detection (2 minutes) and microgram sensitivity bands are not fixed to gel so they can be used for other techniques

What is added to the stacking gel?

Tris-HCl pH 6.8

What is added to the resolving gel?

Tris-HCl pH 8.3

What is a gradient gel?

a gel that can be used in which the acrylamide concentration increases towards teh bottom of the gell

What is 2,2,2-trichloroethanol?

a molecle that will react with tryptophan under UV light

Advantages and disadvantages of silver staining

ad: high sensitivity dis: time consuming, difficult, expensive and has toxic biproducts

How does SDS denature proteins?

by breakng weak interactions and causing the protein to unfold and linearize due to repulsion

Advantages and disadvantages of B-ME

cheaper but more volatile and less potent

Why is the polypeptide chains more negative than normal?

each SDS molecules has 2 negative charges at pH values

How sensitive is SDS PAGE?

enough to resolve between 2 proteins that are approximately 1% apart in mass

Where are the most contaminants found

in the first few lanes

What is SDS PAGE used to determine?

weight, identity, purity and quantity

Can pore size be adjusted any other way?

yes, by adjusting the amount of acrylamide/BIS crosslinking

If proteins of a low weight are being used, the gel should have a ___ % of acrylamide

higher

Size of lysozyme

14 dKa

Which proteins migrate first, large or small?

Small! Large pores can not pass through

What does the pH difference generate?

an ion gradient via glycine and Cl- which carry the current and assist in the stacking process

Ammonium persulfate (APS)

necessary to catalyze the reaction between acrylamdie and BIS

The migration of a protein is

negatively proportional to the log of the proteins mass

What must gels be?

strong, hydrophillic, uncharge , stable and have an adjustable pore size

What would happen if there wasn't stacking gel added?

the gel would be very wide and unreadable

What is logarithmic migraion?

the moleculear weight is closer at the top than the bottom 10 and 15 have the same distance apart as 150 and 250

Electrophoresis

the movement of charged molecules toward and electrode of the opposite charge

What is fixing?

using dyes requires this to fix the protein to the gel via ethanol, methanol or acetic acid to make sure they dont leave teh fel

Autoradiography

most sensitive gel detection that uses radioisotypoes and x-ray film

Once a protein is fixed and bound to a due are they usable with other techniques?

no, normally duplicate gels are made one for staining and one for western blot

Densitometer

used to measure the intensity of bands, which would indicate a relative protein concentration compared to a known marker

Lysozyme weight

14 kDa

Gel electrophoresis

the seperation of charged molecules through a gel matrix in order to sort them by size or charge

What is the stacking gel?

5% acrylamide cast on top of resolving gel and contains wells proteins samples will be loaded into

Size of BSA

67 kDa

What is the counterion?

glycine

What kind of chemicals can break disulfide bridges?

B-ME or dithiothreitol

What is bromophenol blue?

a small, negatively charged molecule that gives the protein sample a blue color

What types of isotypes can be used?

35S, 32P, 33P, 14C and 3H

What is a loading control?

like beta-actin, can be used for normalization to account for variations in pipetting between lanes after gel is tained

What does the dominate SDS charge cause?

separation of denatured, detergent-coated polypeptide chains will be due almost exclusively to the difference in sizes of the polypeptide chains and not the difference in charges

Are oligomers broken during this process?

yes

What is silver staining

10-100x more sensitive than coomassie, offers nanogram detection where silver atoms bind tightly to proteins and produce black or purple bonds

Resolving gel

10-15% acrylamide gel undeneath the stacking gel

Charge to mass ratio

0.5

What is the SDS ratio?

1 SDS molecule per 2 amino acids

Will disulfide bridges be broken in this process of adding a sample loading buffer?

No! they must be broken with special chemicals

What is SDS PAGE?

Sodium dodecyl sulfate polyacrylamide gel electrophoresis

What is a sample loading buffer

addition of SDS, beta-mercaptoethanol, bromophenol blue and glycerol to the protein sample

What do newer coomassie blue agents do?

allo the bands to be viewed directly during staining

Why would multiple bands show up in one lane?

because they are different modifications of the band

What does sodium dodceyl sulfate do?

binds to amino acids and coats proteins in an overwhelming negative charge

Acrylamide will only polymerize

into long chains so the cross linking agent N,N' methylene bisacrylamide is necessary to generate pores

Why is glycerol added to the sample?

it makes the samples more dense than the running buffer and ensures they sink into the wells

SDS PAGE seperates based on?

molecular weight alone

What does polyacrylamide gel do?

prevent loss of resolution caused by diffusion and vibrational and convectional disturbances and allows one to retain the seperation of different proteins after completion of eh experiment

Tetramethylethylenediamine (TEMED)

radicals induce cross linking and polymerize acrylamide and BIS

Relative mobility

ratio of distance each protein migrate to the that of tracking dye

Which gel preforms the seperation of proteins?

resolving gel

The seperation of proteins gel electrophoresis is influenced by

size of the proteins and charge of proteins at the buffer pH

More acrylamide = ___ pores and ____ migration

slower migration and smaller pores

Acrylamide

small molecule that will polymerize into chains under the right condition and the porosity of teh polymerized polyacrylamide gel can be controlled

What is pore size determined by?

the concentration of acrylamide

What part of the gel is used for tracking distance?

the top of teh gel

What happens after a sample loading buffer is added?

they are heat to near boiling to denature proteins. The detergent and heat dirsupt weak bonds

How can the bands on gels be fixed?

they can be dried in cellophane and taped to a lab notebook

What is the a common visualizing agent for protein on gel?

tightly binding dyes like coomassie brilliant blue

Disadvantages to autoradiography

time consuming and requires special certifications

The first few lanes contain

what was loaded, flowthrough and wash


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