Western Blot Protocol

2015-03-02

azim58 - Western Blot Protocol

See also


Western Blot Protocol
Here's the original protocol I received: Western Blot Protocols.pdf
Here's some Western Blot Images

Introduction:
A Western Blot is an analytical technique that is used to detect specific
proteins. It is a process that starts with SDS/Page gel electrophoresis
which separates denatured proteins by their size. Once separated, the
proteins are transferred to a nitrocellulose membrane where they are
probed using antibodies specific to the protein of interest.

Equipment:
Pipettes
Heating block
Centrifuge
XCell4 SureLock™ Midi-Cell Runner (Invitrogen, Cat# WR0100)
Mic;li-Trans Blot Electrophoretic Transfer Cell (Bio-Rad, Cat # 170-3930)
Power Supply (Bio-Rad, Cat # 164-5050)
Incubator, 5% CO2, 3rC

Materials:
Ladder/Marker

o Last seen in yellow box in door of -20 freezer by autoclave

SDS 4x Loading dye (BioRad, Cat# NP0007)
2-mercapotethanol (Sigma, Cat# M7154)
4-12% Bis-Tris NuPAGE Novex Precast Gel (Invitrogen, Cat # WG1403BOX)
1x Tris/Glycine/SDS Electrophoresis Buffer, dilute from 10X (Bio-Rad Cat#
161-0772EOU)
1x Transfer Buffer-
100mL 10X Transfer Buffer (Glycine, Tris Base), 200mL Methanol, up to
1000mL with molecular grade
water. or
1 L 1 x Transfer buffer recipe:
14.4 g
  1. 02 g
20%
GlYCine Electrophoresis Grade (MP Biomedicals, Cat # ICN808822)
Tris Base Electrophoresis Grade (Fisher Scientific, Cat # BP152-500)
Methanol (Fisher Scientific, Cat # A412-1)
Blotting Sandwich (Bio-Rad, Cat# 162-0235)
Vacutainer (BO, Cat # 8304250)

Procedures:
Polyacrylamide Gel

Samples are run alongside a ladder (often 4 uL).
o Running buffer recipe per sample: 2.5 uL loading reagent (80%
dye; 20% mercaptoethanol reducing agent), 1 uL Sample, 7.5 uL 1 x MES
Buffer, 10 uL total volume.
- different volumes can be used as well of course
- The MES is not necessary. The sample can be diluted directly
with 4X loading reagent.
- A western blot can detect about 100 ng protein or less


heat bath. Spin down vial prior to opening and loading gel.
at bottom of gel. Gel wells should be facing in. Load empty block into
back slot if two gels are not being run.
buffer so that buffer fills up the inside of the compartment and
probably about half-way up the outside of the compartment. Load the
ladder as well (4 uL)
silver stain (a coomassie stain or silver stain (more sensitive) will
detect all of the proteins present, whereas the antibody probing of a
Western will detect specific proteins) and one for the nitrocellulose
membrane)
o Samples are transferred to a nitrocellulose membrane via a wet
transfer method.
o Use ice cold transfer buffer. Transfer buffer can be made and
reused up to 3x before discarding.
o Assembly of the Transfer Cassette-
o Remove the gel from the precast assembly and suspend in a tray of
transfer buffer.
o Handling Notes: All 'pre-wet" components are pre-wet with ice
cold transfer buffer. Ensure to keep all components wet during
assembly, do not allow drying to occur.
o Cassette Assembly-BioRad


Make sure to roll out bubbles.
Black Electrode-
Black Cassette Back
Pre-wet Sponge
Pre-wet filter paper (-4.0mm)
Polyacrylamide gel
Pre-wet nitrocellulose membrane with shiny side touching gel
(alternatively PVDF membrane can be used but must be soaked in methanol.
Even then though the nitrocellulose is better from what I understand)
(Using wet filter paper above NC membrane roll out bubbles and then
continue with assembly)
Pre-wet filter paper (-4.0mm)
Pre-wet Sponge
Clear. Cassette front
Red Electrode



o Insert assembled transfer cassette into the rig with ice block and
fill with transfer buffer to the top of the cassette.
o Run at 60V for 60 min
o During transfer, process can be checked by unplugging the transfer
rig and opening the cassette and pealing the corner of the filter paper
back to view the membrane. If the transfer requires more time, the rig
can be reassembled and plugged back in to continue for additional 5-10
min increments.
o Placing the transfer rig in an ice bucket with crushed ice will
further ensure it does not overheat.
o You may want to do a coomassie stain on one of the gels or part of a
gel to detect all of the proteins present, whereas the antibody probing
will detect specific proteins.

o Remove the membrane from the assembly with forceps and transfer
directly into 1 % BSA in TBST.. You may want to cut the bottom right
corner of front to keep track of the orientation.
o Incubate at 4° C overnight or 30 min - 2 hr room temperature.


o Antibody is diluted 1 :1,000 in 5% BSA in TBST (often 20 uL in 20
mL)
o Membrane is incubated in Primary Antibody Solution for 1-2 hrs at
room temp while rotating
o Wash 3X with TBST (may want to wash on rocker for 5 min intervals)


o Dilute biotinylated secondary antibody 1:10,000 in 5% BSA in TBST
(often 2 uL in 20 mL)
o Incubate membrane with antibody for 1 hour
o Wash 3X with TBST (may want to wash on rocker for 5 min intervals)


o Dilute streptavidin dye 1:10,000 in 5% BSA in TBST (often 2 uL in
20 mL)
o Incubate membrane with antibody for 1 hour in the dark
o Wash 3X with TBST (may want to wash on rocker for 5 min intervals)
o Dry membrane (it can be dried faster by pressing between two dry
sponges; may want to dry for 10-20 min)


o Turn on the computer for the Typhoon and select the Typhoon
Scanner icon.
o Set to fluorescence
o Click Setup
o Deselect laser options
o Select the appropriate Emission and excitation lasers
o Last Settings used were: Excitation: 633 nm, Emission filter: 670
nm, Dye: AF647
o May want to reduce the PMT to 350
o Orient membrane on scanner
o Select blocks to scan and click "scan"
o Ensure to save file on server or flash drive instead of on the
computer or the file will be deleted later. Note that the standard
.gel files do not open well in other programs so make sure to at
least save a .tif file.