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Using a Western blot, we will evaluate at what level our lab stock of HEK293 cells express Syk relative to the amount of Syk we plan to introduce as part of our BCR Tango system.

Knowing whether or not our HEK293 cells express Syk will better enable us to determine what level of Syk expression we need in our HEK293 model system and how much cross-talk we can expect from recruitment of endogenous Syk to the BCR upon antigen binding.

Part
pEXPR TRE: Syk-TEV (or pEXPR TRE: Syk-eYFP)
anti-Syk antibodies + secondaries
anti-GADPH antibodies + secondaries

Transfection

Well 1

HEK293

Well 2

B-Cells

Well 3

HEK293

Dummy DNA 1000 ng

Well 4

HEK293

hEF1a: YFP 400 ng

Dummy DNA 600 ng

Well 5

EMPTY

Well 6

EMPTY

Well 7

HEK293

hEF1a: YFP 400 ng

hEF1a: rtTA 200 ng

TRE: Syk-TEVp 400 ng

0 nM Dox

Well 8

HEK293

hEF1a: YFP 400 ng

hEF1a: rtTA 200 ng

TRE: Syk-TEVp 400 ng

1 nM Dox

Well 9

HEK293

hEF1a: YFP 400 ng

hEF1a: rtTA 200 ng

TRE: Syk-TEVp 400 ng

10 nM Dox

Well 10

HEK293

hEF1a: YFP 400 ng

hEF1a: rtTA 200 ng

TRE: Syk-TEVp 400 ng

100 nM Dox

Well 11

HEK293

hEF1a: YFP 400 ng

hEF1a: rtTA 200 ng

TRE: Syk-TEVp 400 ng

1000 nM Dox

Well 12

HEK293

hEF1a: YFP 400 ng

hEF1a: rtTA 200 ng

TRE: Syk-TEVp 400 ng

2000 nM Dox

Gels:

We have the any kD gels in the lab (expire 2015) and this will work for both our western blot and antibody group's western blot.

If we run out of the above gel we are considering getting the 4-25% gel in order to optimize our resolution. This will also work for both our western blot and antibody group's western blot.

The gels currently in the lab have 10 lanes. Here is the plan for the gel:

Lane 1

Lane 2

Lane 3

Lane 4

Lane 5

Lane 6

Lane 7

Lane 8

Lane 9

Lane 10

Ladder

Well 2

B-cells

Well 3

HEK293

Dummy DNA 1000 ng

Well 4

HEK293

hEF1a: YFP 400 ng

Dummy DNA 600 ng

Well 7

HEK293

hEF1a: YFP 400 ng

hEF1a: rtTA 200 ng

TRE: Syk-TEVp 400 ng

0 nM Dox

Well 8

HEK293

hEF1a: YFP 400 ng

hEF1a: rtTA 200 ng

TRE: Syk-TEVp 400 ng

1 nM Dox

Well 9

HEK293

hEF1a: YFP 400 ng

hEF1a: rtTA 200 ng

TRE: Syk-TEVp 400 ng

10 nM Dox

Well 10

HEK293

hEF1a: YFP 400 ng

hEF1a: rtTA 200 ng

TRE: Syk-TEVp 400 ng

100 nM Dox

Well 11

HEK293

hEF1a: YFP 400 ng

hEF1a: rtTA 200 ng

TRE: Syk-TEVp 400 ng

1000 nM Dox

Well 12

HEK293

hEF1a: YFP 400 ng

hEF1a: rtTA 200 ng

TRE: Syk-TEVp 400 ng

2000 nM Dox

Since Syk-TEVp should run at a different band size than endogenous Syk, we should be able to identify the presence of both or either on a Western blot using anti-Syk antibodies. (There should be two bands, one corresponding to Syk-TEVp and the other to endogenous Syk.) We can use GAPDH (which we assume is produced at the same level in all of the cell populations we are testing) to normalize our data. This way, we can make comparisons between different cell populations while controlling for the amount of protein that we loaded in each lane. After washing the paper blot with anti-Syk and anti-GADPH, we should get three bands based on the sizes of the proteins:

Protein	Size (kDa)
Syk	72.08
Syk-(15aa)-TEVp	100.5
GAPDH	37
GFP	27

GFP is added to control for variations in transfection efficiency for each transfection in the dox ladder. From the intensity of these bands, we should be able to determine the relative levels of endogenous and exogenous Syk expression.

Lysis buffer (from Abcam)

pH 8.0

150 mM NaCl

10% NP40 or Triton X-100

50 mM Tris

Running buffer (from Bio-Rad)

pH 8.3

25 mM Tris

192 mM glycine

0.1% SDS

Gel stain

0.3 M CuCl₂

Gel destaining buffer

pH 8.0

0.25 M Tris

0.25 M EDTA

Transfer buffer

48 mM Tris

39 mM glycine

0.04% SDS

20% methanol

TBST (Antibody/BSA buffer)

100 mL TBS 10x (pH 7.6)

24.23 g Trizma HCl
80.06 g NaCl
to 1L with dH₂O

900 mL dH₂O

1 mL Tween20