SDS/PAGE Flashcards

1
Q

What is the separation in SDS-PAGE based on?

A

Movement of charged proteins in an electrical field and sieving effects

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2
Q

What is SDS/PAGE an analytical tool for?

A
  • Determining the purity of protein preparations
  • Approximate molecular weight determination
  • Western blot analysis
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3
Q

What is the migration of proteins approximately proportional to?

A

Their mass

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4
Q

Which molecules will have greater mobility with same charge density?

A

Small

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5
Q

How can proteins be visualized?

A

1) Staining (e.g., Coomassie or silver ions) - all proteins
2) Chemiluminescence - Antibody-based detection - specific target protein

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6
Q

What are the titles for the x- and y-axis when determining the concentration of an unknown protein?

A

x - relative migration
y - logMr

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7
Q

What are the objectives of this lab?

A
  • Efficient casting of SDS-PAGE gels
  • Proper sample application and gel running
  • Visualization of proteins by Coomassie staining
  • Analysis of successful E. coli expression of PTEN (IPTG induction success; cell lysis efficiency; solubility analysis)
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8
Q

What does proteomics aim to identify?

A

The protein complement of a particular cellular state

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9
Q

What is proteomics useful for?

A
  • Deciphering organelle-specific protein
  • Mapping functional networks
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10
Q

What was a biomarker discovery of proteomics?

A

Differential expression analysis

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11
Q

How can gel electrophoresis be employed within proteome studies?

A

As a separation step to reduce sample complexity and visualize potential biomarkers

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12
Q

How is protein separated in 2D gel electrophoresis?

A

Weight and isoelectric point

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13
Q

What does 2D gel electrophoresis combine to give?

A

Combines isoelectric focusing and SDS-PAGE to give a fingerprint of protein expression in a given cell

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14
Q

What happens in the first dimension of 2D gel electrophoresis?

A

Isoelectric focusing gel with decreasing pI is placed on SDS polyacrylamide gel

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15
Q

What happens in the second dimension of 2D gel electrophoresis?

A

SDS polyacrylamide gel electrophoresis with decreasing Mr from top to bottom and decreasing pI from left to right

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16
Q

What is DIGE?

A

Difference gel electrophoresis - quantifying technique for protein purification

17
Q

How is DIGE carried out to overcome non-biological variation?

A

1) Label protein extracts using CyDye DIEGE Fluor minimal dyes
2) Mix labelled extracts
3) 2D separation
4) Image gel with CyDye specific scanner (scan at different wavelengths)
5) Image analysis and data quantitation using appropriate software

18
Q

What are the advantages of fluorescent detection?

A
  • Increased dynamic range
  • Spot co detection
  • Accurate (corresponding spots have the same boundary, ensuring exact spot volume rations)
19
Q

What is the proteomics 2D gel-based workflow?

A

1) Sample prep
2) Sample loading
3) Protein separation
4) Image acquisition
5) Image analysis
6) Automated spot picking
7) Spot digestion
8) MALDI target spotting
9) Spot handling workstation

20
Q

In a scientific report, what did chronic stepwise cerebral hypoperfusion do?

A

Differentially induced synaptic proteome changes in the frontal cortex, occipital cortex, and hippocampus in rats