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Expand
titleTest 2
Expand
titleDescription

Use anti IgM with a fluorescent fused secondary antibody to test for membrane localization of the BCR complex. Use B-Cells as a control.

Expand
titlePurpose

This will test whether or not the BCR complex will reach the cell membrane in HEK293 cells.

Expand
titleParts Needed

pEXPR hEF1a: Gmab Light

pEXPR hEF1a: Gmab Heavy

pEXPR hEF1a: CD79A

pEXPR hEF1a: CD79B

ALSO NEED:

Anti IgM primary antibody fused to a yellow alexa dye

B cells

Expand
titleSetup

PLATE 1

Well 1

B-Cells

Well 2

HEK293

Well 3

HEK293

Well 4

HEK293

mKate 200 ng

Dummy DNA 800 ng

Well 5

HEK293

Gmab L 200 ng

Gmab H 200 ng

CD79A 200 ng

CD79B 200 ng

mKate 200 ng


Well 6

B-Cells

Well 7

B-Cells

Well 8 

HEK293

Well 9

HEK293

Well 10

HEK293

mKate 200 ng

Dummy DNA 800 ng


Well 11

HEK293

Gmab L 200 ng

Gmab H 200 ng

CD79A 200 ng

CD79B 200 ng

mKate 200 ng

 

Well 12

B-Cells

Well 13 

B-Cells

Well 14 

HEK293

Well 15

HEK293

Well 16

HEK293

mKate 200 ng

Dummy DNA 800 ng

 

Well 17

HEK293

Gmab L 200 ng

Gmab H 200 ng

CD79A 200 ng

CD79B 200 ng

mKate 200 ng

 

Well 18

B-Cells

Well 19 

B-Cells

Well 20

HEK293

Well 21

HEK293

Well 22

HEK293

mKate 200 ng

Dummy DNA 800 ng

 

Well 23

HEK293

Gmab L 200 ng

Gmab H 200 ng

CD79A 200 ng

CD79B 200 ng

mKate 200 ng

 

Well 24

B-Cells

PLATE 2

Well 1

B-Cells

Well 2

HEK293

Well 3

HEK293

Well 4

HEK293

mKate 200 ng

Dummy DNA 800 ng

Well 5

HEK293

Gmab L 200 ng

Gmab H 200 ng

CD79A 200 ng

CD79B 200 ng

mKate 200 ng


Well 6

B-Cells

Well 7

B-Cells

Well 8 

HEK293

Well 9

HEK293

Well 10

HEK293

mKate 200 ng

Dummy DNA 800 ng


Well 11

HEK293

Gmab L 200 ng

Gmab H 200 ng

CD79A 200 ng

CD79B 200 ng

mKate 200 ng

 

Well 12

B-Cells

EMPTY

EMPTY

EMPTYEMPTYEMPTYEMPTY
EMPTYEMPTYEMPTYEMPTYEMPTYEMPTY
Expand
titleExpected Results

We expect to see clear yellow fluorescence around the blue stained nuclei indicating BCR localization to the HEK cell membrane. Moreover Transfection efficiency as measured by our mKate transfection marker should correlate to anti IgM fluorescence in the flow cytometer. B-Cells should act as a positive control for this experiment.

Expand
titleProtocol

calibrate cytometer with wells2/8

then run remaining tubes sequentially

image well 1 b-cells alt 7

image well 3 stained HEK293 cells with no DNA alt 9

image well 4 stained HEK293 cells withmkate + Dummy DNA alt 10

image well 5 stained HEK293 with BCR alt 11

image well 13 permeablized b-cells alt 19

image well 15 permeablized HEK293 with no DNA alt 21

image well 16 permeablized HEK293 with mkate+dummy alt 22

image well 17 permeablized HEK293 with BCR alt 23

Expand
titleData

 

Expand
titleAnalysis

 

Expand
titleTest 2
Expand
titleDescription

Use anti IgM with a fluorescent fused secondary antibody to test for membrane localization of the BCR complex. Use B-Cells as a control.

Expand
titlePurpose

This will test whether or not the BCR complex will reach the cell membrane in HEK293 cells.

Expand
titleParts Needed

pEXPR hEF1a: Gmab Light

pEXPR hEF1a: Gmab Heavy

pEXPR hEF1a: CD79A

pEXPR hEF1a: CD79B

ALSO NEED:

Anti IgM primary antibody fused to a yellow alexa dye

B cells

Expand
titleSetup

PLATE 1

Well 1

B-Cells

Well 2

HEK293

Well 3

HEK293

Well 4

HEK293

mKate 200 ng

Dummy DNA 800 ng

Well 5

HEK293

Gmab L 200 ng

Gmab H 200 ng

CD79A 200 ng

CD79B 200 ng

mKate 200 ng


Well 6

B-Cells

Well 7

B-Cells

Well 8 

HEK293

Well 9

HEK293

Well 10

HEK293

mKate 200 ng

Dummy DNA 800 ng


Well 11

HEK293

Gmab L 200 ng

Gmab H 200 ng

CD79A 200 ng

CD79B 200 ng

mKate 200 ng

 

Well 12

B-Cells

Well 13 

B-Cells

Well 14 

HEK293

Well 15

HEK293

Well 16

HEK293

mKate 200 ng

Dummy DNA 800 ng

 

Well 17

HEK293

Gmab L 200 ng

Gmab H 200 ng

CD79A 200 ng

CD79B 200 ng

mKate 200 ng

 

Well 18

B-Cells

Well 19 

B-Cells

Well 20

HEK293

Well 21

HEK293

Well 22

HEK293

mKate 200 ng

Dummy DNA 800 ng

 

Well 23

HEK293

Gmab L 200 ng

Gmab H 200 ng

CD79A 200 ng

CD79B 200 ng

mKate 200 ng

 

Well 24

B-Cells

PLATE 2

Well 1

B-Cells

Well 2

HEK293

Well 3

HEK293

Well 4

HEK293

mKate 200 ng

Dummy DNA 800 ng

Well 5

HEK293

Gmab L 200 ng

Gmab H 200 ng

CD79A 200 ng

CD79B 200 ng

mKate 200 ng


Well 6

B-Cells

Well 7

B-Cells

Well 8 

HEK293

Well 9

HEK293

Well 10

HEK293

mKate 200 ng

Dummy DNA 800 ng


Well 11

HEK293

Gmab L 200 ng

Gmab H 200 ng

CD79A 200 ng

CD79B 200 ng

mKate 200 ng

 

Well 12

B-Cells

EMPTY

EMPTY

EMPTYEMPTYEMPTYEMPTY
EMPTYEMPTYEMPTYEMPTYEMPTYEMPTY
Expand
titleExpected Results

We expect to see clear yellow fluorescence around the blue stained nuclei indicating BCR localization to the HEK cell membrane. Moreover Transfection efficiency as measured by our mKate transfection marker should correlate to anti IgM fluorescence in the flow cytometer. B-Cells should act as a positive control for this experiment.

Expand
titleProtocol

calibrate cytometer with wells2/8

then run remaining tubes sequentially

image well 1 b-cells alt 7

image well 3 stained HEK293 cells with no DNA alt 9

image well 4 stained HEK293 cells withmkate + Dummy DNA alt 10

image well 5 stained HEK293 with BCR alt 11

image well 13 permeablized b-cells alt 19

image well 15 permeablized HEK293 with no DNA alt 21

image well 16 permeablized HEK293 with mkate+dummy alt 22

image well 17 permeablized HEK293 with BCR alt 23

Expand
titleData

 

Expand
titleAnalysis