Western blotting of XK and VPS13A

Pietro De Camilli, Chase Amos

Published: 2023-12-14 DOI: 10.17504/protocols.io.3byl4qb6zvo5/v1

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Abstract

This protocol describes collection of protein from cultured cells and immunoblotting.

Steps

Cell culture and treatments

Culture K562 or COS-7 (ATCC) at 37°C and 5% CO2, using RPMI for K562 or DMEM for COS-7 containing 10% FBS, 1millimolar (mM) sodium pyruvate, 100 penicillin, 100 streptomycin, 2millimolar (mM) L-glutamine, 1 non-essential amino acids, (all from Gibco) and 2.5 plasmocin (InvivoGen).

For K562 cells treated with hemin, supplement the media with hemin (Sigma Aldrich) dissolved in DMSO to a final concentration of 30micromolar (µM) for 48h 0m 0s .

Cell lysis and sample preparation

Prior to K562 lysis, pellet the cells by centrifuging at 1100rpm,4°C . Resuspend the pellet in PBS, centrifuging and repeating for a total of 3 times.

3.1.

Resuspend in PBS and centrifuge 1100rpm,4°C (1/3).

3.2.

Resuspend in PBS and centrifuge 1100rpm,4°C (2/3).

3.3.

Resuspend in PBS and centrifuge 1100rpm,4°C (3/3).

Prior to lysis of confluent COS-7 cells, aspirate media and wash with PBS 3 times.

Lyse cells with 2% SDS by either resuspending (K562) or adding to culture dish and scraping using a Corning cell-lifter (COS-7). Sonicate lysates using 3x10s pulses with Virsonic 550 (Virtis).

Centrifuge 13300rpm and collect the post-nuclear supernatant in a new Eppendorf tube.

Determine protein concentration in sample using Pierce BCA assay (ThermoFisher).

Prepare samples at desired concentration and add SDS loading buffer to reach a final concentration of 50millimolar (mM) 06.8 Tris, 2Mass / % volume SDS, 0.1Mass / % volume bromophenol blue, 10% (v/v) glycerol, and 1% (v/v) beta-mercaptoethanol.

Boil 95°C for 0h 10m 0s .

Gel electrophoresis and immunoblotting

10.

Prepare gel apparatus with 4-12% Tris Glycine gels (Invitrogen) and Tris-Glycine SDS running buffer.

11.

Load samples into gel and run until dye front reaches bottom (120-150 V).

12.

Remove gel and set up transfer cassette with nitrocellulose membrane.

13.

Transfer at 30 V at 4°C in NuPage transfer buffer (Invitrogen)

14.

Remove nitrocellulose membrane and block membrane with 5% BSA in TBST for 1h 0m 0s at 22Room temperature .

15.

Add primary antibodies at desired concentration in 5% BSA in TBS-T, incubate at 4°C .

16.

Wash membrane with TBST. Repeat a total of 3 times.

16.1.

Wash membrane for 0h 5m 0s with TBST (1/3).

16.2.

Wash membrane for 0h 5m 0s with TBST (2/3).

16.3.

Wash membrane for 0h 5m 0s with TBST (3/3).

17.

Incubate membrane with secondary antibodies conjugated to IRdye 800CW or IRdye 680CW (1:10,000, Licor) in 5% BSA in TBST for 1h 0m 0s at Room temperature .

18.

Wash membrane with TBST. Repeat a total of 3 times.

18.1.

Wash membrane for 0h 5m 0s with TBST (1/3).

18.2.