Lab 9 Protein Analysis Flashcards

Question 1

Q

Fish fraud is only an economical concern.
True or False?

Answer

A

False.
Cheaper fish species are not always safe for human consumption, so fish fraud is also a food safety concern.

For example, escolar, often sold as white tuna, can cause diarrhea-like symptoms, and amberjack often sold as yellowtail tuna, can have a naturally occurring toxin that causes neurological symptoms.

Question 2

Q

What is ‘crude protein’?

Answer

A

Protein (muscle, myofibrillar, and stroma) and non-protein nitrogen (generally from sarcoplasm)

Question 3

Q

What is PAGE?

Answer

A

Polyacrylamide gel electrophoresis
A technique in which proteins are separated in a cross-linked acrylamide gel matrix.

Question 4

Q

How are proteins separated in SDS-PAGE?

Answer

A

Proteins are denatured using heat, mercaptoethanol, and anionic detergent (SDS)
Separation takes place on the basis of size, since the SDS makes all proteins uniformly negative in charge.

SDS = sodium dodecyl sulfate

Question 5

Q

How are proteins separated in native-PAGE?

Answer

A

Proteins are separated based on their native charge and molecular weight.

Question 6

Q

How are proteins separated in IEF-PAGE?

Answer

A

Native proteins are separated by native charge in a pH gradient.
Each protein migrates until it reaches the pH of its isoelectric point (the point where there is no net charge on the protein).
- Proteins with a net positive charge (below its isoelectric point) will migrate toward the cathode.
- Proteins with a net negative charge (above its isoelectric point) will migrate toward the anode.

IEF = isoelectric focusing

Question 7

Q

In IEF-PAGE proteins with a net positive charge (below its isoelectric point) will migrate toward the cathode.
True or False?

Question 8

Q

In IEF-PAGE proteins with a net positive charge (below its isoelectric point) will migrate toward the anode.
True or False?

Answer

A

False.
In IEF-PAGE proteins with a net positive charge (below its isoelectric point) will migrate toward the cathode.

Question 9

Q

In IEF-PAGE proteins with a net negative charge (above its isoelectric point) will migrate toward the anode.
True or False?

Question 10

Q

In IEF-PAGE proteins with a net negative charge (above its isoelectric point) will migrate toward the cathode.
True or False?

Answer

A

False.
In IEF-PAGE proteins with a net negative charge (above its isoelectric point) will migrate toward the anode.

Question 11

Q

Which type of PAGE is used to authenticate food samples?
How does it work?

Answer

A

IEF-PAGE

The species from which a food sample was obtained can be determined by matching the pattern arising from the protein bands with known standards.
Proteins from different species will have a unique pattern when run on an IEF-PAGE because of different amino acid compositions, even if the molecular weight of the proteins from the two different species are almost identical.

Question 12

Q

You want to conduct a milk protein analysis using a casein protein standard curve. Your standard curve will have 8 points and 3 technical replicates and you will also prepare 3 technical replicates of 2 diluted milk samples. 200 µL of BCA reagent will be added to each sample and standard.

What is the minimum volume of BCA reagent you should prepare?

Question 13

Q

What wavelength do you use when carrying out a BCA assay?

Question 14

Q

What is the principle behind the Bicinchoninic Acid Method protein assay?

Answer

A

Reduction of Cu2+ to Cu1+ by protein in an alkaline solution and the ions will be trapped by two molecules of BCA to create a purple-colored product

Question 15

Q

What is the problem when your protein standard curve is constructed using concentrations 0 – 2.0 mg/ml (with absorbance of 0.134 – 0.843) but the absorbance of your sample is 0.953?

Answer

A

You cannot ensure that the relationship between concentration and absorbance is still linear to extrapolate the result

Question 16

Q

What colour should your BCA working reagent be?

Question 17

Q

In this example:
How much of each standard concentration do you need?
How much of the fish sample do you need?
How much total BCA reagent do you need?

Answer

A

Standard concentration: 10 uL x 3 = 30 uL
Sample: 10 uL x 3 = 30 uL
Reagent: (6 standards + 1 sample) x 200 uL x 3 replicates = 4200 uL

Question 18

Q

Fill in the table – choose 6 equally spaced dilutions between 0 and 2 mg/mL including 0 mg/mL as one of the 6 standards. Prepare 1 mL of each standard

2.0 mg/mL standard

Question 19

Q

Now, let’s prepare 2 dilutions of the fish sample:
* Fish are known to contain between 20 – 30 g protein/100 g of fish
* The protein extraction method requires us to homogenize 25 g of fish in
100 mL of water
* What is the possible protein concentration range in this homogenous solution?

Question 20

Q

Question 21

Q

What is the mechanism of the BCA assay?

Answer

A

Peptide bonds in protein reduce Cu2+ to Cu1+ in the presence of a base
BCA reagent is alkaline (~pH 11)
Temperature-dependent assay!!
Every assay needs a new standard curve
The amount of Cu2+ reduced is proportional to the amount of protein in the sample
BCA reagent chelates the Cu1+ from the protein to form a complex
2 moles of BCA to 1 mole of Cu1+
Not a reaction, no bonds are formed
Creates a colored product that can be quantified at λ = 562 nm

Question 22

Q

The BCA assay involves a reaction between the BCA reagent and copper.
True or False?

Answer

A

False.
No bonds formed.
BCA reagent chelates the Cu+1 (reduced from Cu2+ by peptide bonds in protein) to form a complex

Question 23

Q

The BCA assay is temperature-dependent.
True or False?

Answer

A

True.
Every assay needs a new standard curve.

Question 24

Q

The BCA agent is acidic.
True or False?

Answer

A

False.
It is alkaline.

Question 25

Q

The BCA reagent is alkaline.
True or False?

Question 26

Q

You discovered the casein solution you used to construct a standard curve was actually 1.7 mg/mL, not 2 mg/mL. How will this affect the protein concentration you determine?

Answer

A

Overestimation

Question 27

Q

What happens if the reagent changes from green to purple before adding a protein sample?

Biuret reaction a.k.a. BCA protein assay

Answer

A

Glassware or pipette tips contaminated reagent (very sensitive to metal ions)

Question 28

Q

How do you prepare BCA reagent from reagents A and B?

Answer

A

50 parts A to 1 part B

Question 29

Q

How long is prepared BCA working reagent stable?

Answer

A

For a short duration in a closed container at room temperature

Question 30

Q

Describe the basis of the Kjeldhal method of protein determination.

Answer

A

Determination of the % total nitrogen in a sample
Convert to % protein using a conversion factor that varies with different food matrices.

Question 31

Q

What are the three basic steps of the Kjeldahl method?

Answer

A

Digestion
Neutralization and distillation
Titration

Question 32

Q

What happens during the digestion step of the Kjeldahl method?

Answer

A

Proteins and other organic food components are digested by sulfuric acid in the presence of catalysts.
Protein nitrogen is liberated to form ammonium ions
Carbon and hydrogen elements are converted to carbon dioxide and water.

Question 33

Q

What happens during the neutralization and distillation step of the Kjeldahl method?

Answer

A

Sulfuric acid is neutralized with alkali
The ammonium is distilled into an acid solution

Question 34

Q

What happens during the titration step of the Kjeldahl method?

Answer

A

The % ammonium (or % N) in the solution is determined via back-titration
This value is converted to % protein using the conversion factor that depends on the analyte

Question 35

Q

Why does the Kjeldahl method determine ‘crude protein’ content only?

Answer

A

Nitrogen also comes from nonprotein components (e.g., ammonia and ammonium sulfate)

Question 36

Q

What is the principle by which proteins are separated using SDS-PAGE?

Answer

A

Molecular size

Question 37

Q

What is the principle by which proteins are separated using IEF-PAGE?

Answer

A

isoelectric point

Question 38

Q

What form of acrylamide is toxic to humans?

Answer

A

Unpolymerized

Question 39

Q

Which solution should be added last when preparing the resolving and stacking gels?

Question 40

Q

What is used to flatten down the resolving gel to produce an evenly distributed gel matrix?

Answer

A

Isopropanol

Question 41

Q

What is the purpose of digestion in the Kjeldahl method?

Answer

A

Release ammonium ions from proteins to be indirectly quantified

Question 42

Q

What is the purpose of distillation in the Kjeldahl method?

Answer

A

To convert ammonium ions to ammonia gas

Question 43

Q

What is the purpose of titration in the Kjeldahl method?

Answer

A

Directly quantify total moles of HCl remaining

Question 44

Q

The wells in the SDS-gel should be filled with running buffer before the samples and standard are added.
True or False?

Question 45

Q

The wells in the SDS-gel should be filled with running buffer after the samples and standard are added.
True or False?

Answer

A

False.
The wells in the SDS-gel should be filled with running buffer before the samples and standard are added.

Question 46

Q

What should you do after you have run your SDS gel and removed the glass plates?

Answer

A

Remove the stacking gel

Question 47

Q

What is the difference between stacking gel and resolving gel?

Answer

A

The acrylamide concentration determines the different pore sizes of the polyacrylamide gel. The stacking gel has a lower acrylamide concentration (5%) so the pore size is larger. When an electrical charge is applied to the gel, the proteins move through this part of the gel at a similar speed.
The resolving gel has a higher acrylamide concentration (usually 10 to 15%), meaning it has a smaller pore size than the stacking gel. This part of the gel separates the proteins by their molecular weight. Larger proteins—which have a higher molecular weight—move through the pores in the resolving gel slower than smaller proteins—which have a lower molecular weight.

Question 48

Q

What is Laemmli buffer and what is it used for? [3]

Answer

A

Sample loading buffer or sample dissociation buffer
It contains (1) dye to assist in the monitoring of movement when running a gel.
It also contains (2) SDS, which helps mobilize the proteins in the gel
Lastly, (3) the beta-mercaptoethanol, upon mixing with the sample and heating, reduces disulfide bonds. This reduces multimeric protein down to their constituent proteins

Question 49

Q

What is a running buffer?

Answer

A

Running buffer contains ions that conduct the current being applied through the gel, in turn allowing the proteins (which are covered with SDS, which is charged) to move through the gel.

Question 50

Q

What is the purpose of the Kjeldahl tablets?

Answer

A

The metals in the chemicals act as catalysts.
The K2SO4 (and also sulfate from CuSO4) aids in elevating the boiling point, which allows the liquid phase to get over 100 degrees C and thereby increase the reaction rate/extent.

Question 51

Q

What is the benefit of GelCode blue/Coomassie stains? [2]

Answer

A

They bind all proteins
The staining protocol is streamlined

Question 52

Q

Describe 4 applications of protein electrophoresis.

Answer

A

Protein expression
Molecular weight (MW) of proteins
Presence of certain proteins (via Western blotting with antibodies)
Isolate proteins for mass spectral analysis (cut band of interest out, digest gel, and isolate protein again)

Question 53

Q

Polyacrylamide gels are used to separate proteins.
What is the gel made of?

Answer

A

Acrylamide (A) and bis-acrylamide (B)

Question 54

Q

Polyacrylamide gels are used to separate proteins.
What initiates gel formation?

Answer

A

A free radical (APS) and a free radical stabilizer (TEMED)

APS (ammonium persulfate) and TEMED (tetramethylethylenediamine) are used to initiate the polymerization of acrylamide and a comonomer crosslinker such as bis-acrylamide to form polyacrylamide gels. APS acts as an initiator by decomposing to form free radicals that can initiate polymerization. TEMED acts as a catalyst by accelerating the rate of polymerization.

Question 55

Q

Polyacrylamide gels are porous - which allows for proteins to move through.
What defines pore size?

Answer

A

% acrylamide (as % increases, pore size decreases)
% bis-acrylamide (cross-linker) (as % increases, pore size decreases; minimum pore size occurs at 5% bis-acrylamide)

Question 56

Q

What does the pore uniformity of polyacrylamide gel depend on?

Answer

A

The amount of catalyst (free radical) used
Ammonium persulfate (APS) - free radical source
Tetramethylethylenediamine (TEMED) - helps stabilize the free radicals from the persulfate

Question 57

Q

What is sodium dodecyl sulfate (SDS) used for in protein electrophoresis?

Answer

A

Denatures proteins
Binds them via hydrophobic interactions and imparts a uniform negative charge

Question 58

Q

What is 2-mercaptoethanol used for in protein electrophoresis?

Answer

A

Reduces disulfide bonds allowing for full denaturation/unfolding

Question 59

Q

Describe SDS-PAGE sample preparation.

Answer

A

Protein is uniformly covered in negative charge (~1 SDS per 2 amino acids)
SDS blocks any positive charges on the protein
Regardless of the size of the protein, they all have the same charge:mass ratio

Question 60

Q

Describe the SDS-PAGE set-up.

Answer

A

Cathode (-) at the top
Anode (+) at the bottom

Question 61

Q

Describe protein separation via SDS-PAGE.

Answer

A

Movement of negatively charged proteins through gel pores is due to an applied electric current across the gel.
Rate of movement is inversely proportional to the molecular weight
- Bigger protein = less movement
- Smaller protein = more movement
- Remember: same charge: mass ratio

Question 62

Q

What is a stacking gel?

Answer

A

Low % acrylamide = larger pore size
Does not restrict protein movement by size
Used to align proteins at interphase of two gels in order to achieve accurate separation

Question 63

Q

What is a resolving gel?

Answer

A

Higher % acrylamide = smaller pore size
Used for size separation of proteins

Question 64

Q

Describe how the different gels work together in SDS-PAGE.

Answer 53

A

Binds to proteins through ionic interactions (sulfonic groups on dye and amine groups on protein)
General van der waals interactions
Can detect as little as 0.1 ug of protein

Answer 54

A

Pro: can detect as little as 1 ng of protein (100x more sensitive than Coomassie)
Con: lengthy procedure, reagents used interfere with downstream analyses such as mass spectrometry)

Answer 55

A

Standards of known molecular weight must be run on every gel
Movement of ladder standards will vary with gel preparation and electrophoresis conditions.

Answer 56

A

Extract relative migration of standards and plot log(MW) versus. migration
Standard curve then used to determine molecular weight of unknown proteins or to identify proteins

Answer 57

A

separation based on the isoelectric point (pl) of a protein)

Answer 58

A

Gel is a lower % polyacrylamide gel; does not restrain the movement of proteins by size
Uses a pH gradient gel
Above its pI, a protein is negatively charged and will migrate towards the anode (+)
Below its pI, a protein is positively charged and will migrate towards the cathode (-)
Proteins migrate until they reach their pI’s
No net charge and therefore does not move further

Answer 59

A

Established using ampholytes, that is: small molecular weight molecules that possess both acidic and basic functional groups and form pH gradients under the influence of electric fields

Answer 60

A

Standards of known pI must be run on every gel
Results reported as relative distance travelled from cathode

Answer 61

A

1) Digestion
* Proteins and other organic materials are broken down by sulfuric acid
* Protein nitrogen is released in the form of ammonium ions (NH4+)

2) Neutralization and distillation
* NaOH is added to convert NH4+ to NH3 (gas)
* NH3 is distilled (separated) into an acid solution (HCl)

3) Titration
* NH3 neutralizes some of the HCl
* Remaining HCl is then back-titrated (with NaOH) to determine how much ammonium was present
* %N is then determined and converted to % protein by a conversion factor (food specific)

Answer 62

A

In SDS-PAGE, mercaptoethanol is used as a reducing agent to break disulfide bonds which can form between cysteine amino acids in some proteins. This reduction of disulfide bonds is important for allowing the protein to become completely unfolded so that it migrates properly for its molecular weight.

Answer 63

A

Anionic detergents such as SDS (sodium dodecyl sulfate) are used in SDS-PAGE (sodium dodecyl sulfate polyacrylamide gel electrophoresis) for protein solubilization, linearization and for establishing a uniform charge in preparation for gel electrophoresis. SDS binding denatures the polypeptides and imparts a negative charge that masks their intrinsic charge.

Answer 64

A

Because if the MW of proteins of some species may be almost identical and hard to differentiate.
IEF-PAGE can discern between them because of different amino acid compositions

Answer 65

A

False.
The Kjeldahl method is more precise.

Answer 66

A

True.
The Kjeldahl method is more precise.

Answer 67

A

Tris buffer is used in the preparation of SDS-PAGE gels to maintain a stable pH during the electrophoresis process. The pH of the buffer affects the overall charge of the proteins being separated, which in turn affects their migration through the gel. Tris buffer is commonly used because it has a high buffering capacity and can maintain a stable pH over a wide range of temperatures. This helps to ensure consistent and reproducible results in SDS-PAGE experiments.

Answer 68

A

BCA assay can be affected by interfering substances, variations in protein composition, and temperature. It is also an indirect method that relies on reduction of copper ions by protein in an alkaline solution.
The Kjeldahl method is a direct measurement of nitrogen content.

Answer 69

A

SDS (sodium dodecyl sulfate): a detergent that denatures the proteins and gives them a uniform negative charge, allowing them to be separated based on their size.
Reducing agents (β-mercaptoethanol): these break disulfide bonds within and between protein molecules, further denaturing the proteins.
Glycerol: increases the density of the sample, allowing it to sink to the bottom of the well when loaded onto the gel.
Bromophenol blue: a tracking dye that allows you to monitor the progress of the electrophoresis.

Answer 70

A

The fixing solution (20% TCA) is used after the electrophoresis step to fix the proteins in place within the gel. This is done by crosslinking the proteins to the gel matrix, preventing them from diffusing out of the gel during subsequent steps. The fixing solution typically contains a mixture of alcohols (such as methanol or ethanol) and an acid (such as acetic acid) that help to dehydrate and shrink the gel, further immobilizing the proteins.

The washing solution (30% MeOH: 10% acetic acid: 60% DDH2O) is used after the fixing step to remove any excess fixing solution and unbound proteins or other contaminants from the gel. This helps to improve the clarity and resolution of the final stained gel. The washing solution typically contains water or a mild buffer to gently rinse the gel without disrupting the fixed proteins.

In summary, the fixing solution is used to immobilize the proteins within the gel, while the washing solution is used to remove any excess reagents and contaminants from the gel.

Answer 71

A

Solution changes from pink to orange

Answer 72

A

OPA (o-phthaldialdehyde) reacts with primary amino groups in the presence of 2-ME to form a highly fluorescent isoindole derivative. The 2-ME reduces the OPA molecule, allowing it to react with the primary amino group to form the fluorescent product.

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Lab 9 Protein Analysis Flashcards

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