Practical 2 Flashcards

1
Q

What technique was used first to identify mw of the glut 4 in each sample

A

Sds page

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2
Q

How would you get cytoplasmic and plasma membrane fractions of glut 4 from adipocytes

A

Centrifugstuon of the wt and mutant adipocytes

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3
Q

Why wouldn’t glut4 be seen in membrane with adipocytes mutant

A

Loss of pkc signalling from insulin means glut 4 can’t travel to membrane

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4
Q

Which sample will have the lowest intensity of protein in western blot

A

Cytoplasmic wt with insulin - all the glut 4 goes to membrane

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5
Q

What is in the sds loading gel x 10

A
Glycerol 
Sds 
Dtt 
EDTA metal chelator
Dye
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6
Q

What further denatures proteins in sds

A

Heat

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7
Q

What type of membrane was the gel pressed onto via western blot

A

Nitrocellulose

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8
Q

What type of buffer was used to add each layer on western blot

A

Transfer buffer

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9
Q

What is blocking buffer/agent

A

Something with milk powder or casein in it , it fills the empty protein binding spaces on the membrane so pa and sa don’t non specifically bind

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10
Q

As well as casein what was in blocking buffer

A

Tbst (with tween 20)

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11
Q

What was wash buffer with tbst tween 20 for

A

Wash non specific protein binding from the membrane

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12
Q

Which enzyme was the sa conjugated with

A

Alkaline phosphatase

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13
Q

What was the developer solution

A

The chromogenic substrate added to alkaline phosphatase

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14
Q

What is the product called between the alkaline phosphatase and the chromogenic substrate picked up on western blot

A

Chemiluminescent product

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15
Q

What would more than 1 band on western blot indicate

A

Non specific binding of ab to another protein on membrane

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