ENCAB000AIM

Antibody against Homo sapiens MAZ, Mus musculus MAZ

Homo sapiens

HeLa-S3, GM12878, K562, MCF-7, A549

characterized to standards with exemption

Homo sapiens

any cell type or tissue

partially characterized

Mus musculus

any cell type or tissue

partially characterized

Homo sapiens

HepG2

not characterized to standards

Status: released
Source (vendor): Abcam
Product ID: ab85725
Lot ID: GR41711-2
Characterized targets: MAZ (Homo sapiens), MAZ (Mus musculus)
Host: rabbit
Clonality: polyclonal
Purification: affinity
Antigen description: Immunogen is synthetic peptide, corresponding to a region within amino acids 427-477 of Human MAZ, GenBank BAA33064.1.
External resources: AR:AB_1861254
UCSC-ENCODE-cv:MAZ_(ab85725)

Characterizations

Method: immunoprecipitation

Attachment PDF Icon

not reviewed

Submitted by: Michael Snyder
Lab: Michael Snyder, Stanford
Grant: U54HG004558
Download: human_MAZ_ab85725_validation_Snyder.pdf

Method: immunoprecipitation followed by mass spectrometry

Attachment PDF Icon

not reviewed

Submitted by: Michael Snyder
Lab: Michael Snyder, Stanford
Grant: U54HG004558
Download: human_MAZ_ab85725_validation_Snyder.pdf

HeLa-S3

Method: immunoprecipitation

compliant

Caption: B. Immunoprecipitation of Maz from HeLa-S3 cells using ab85725. Lane 1: input nuclear lysate. Lane 2: unbound material from immunoprecipitation with ab87525. Lane 3: material immunoprecipitated with ab85725. Lane 4: material immunoprecipitated using control IgG. Arrows indicate band at expected size of Maz, and * indicates band of similar intensity and unexpected size (identified as Maz by mass spectrometry).
Submitted by: Kathrina Onate
Lab: Michael Snyder, Stanford
Grant: U54HG004558
Download: IP Snyder AIM.png
Documents: encode:Antibody_Characterization_ENCODE3_August2015.pdf

K562

Method: immunoprecipitation

compliant

Caption: Immunoprecipitation of Maz from K562 cells using ab85725. Lane 1: input nuclear lysate. Lane 2: material immunoprecipitated with ab85725. Lane 3: material immunoprecipitated using control IgG. Bands A and B were excised from the gel and subject to analysis by mass spectrometry.
Reviewer comment: What is the expected band size?
Submitted by: Kathrina Onate
Lab: Michael Snyder, Stanford
Grant: U54HG004558
Download: IP-MS_MAZ:K562 Snyder AIM.png
Documents: encode:Antibody_Characterization_ENCODE3_August2015.pdf

A549

Method: immunoprecipitation

compliant

Caption: Immunoprecipitation was performed on nuclear extracts from the cell line: A549 using the antibody ab85725. The image shows western blot analysis of input, flowthrough, immunoprecipitate, and mock immunoprecipitate using IgG. Target molecular weight: 48.608.
Submitted by: Nathaniel Watson
Lab: Michael Snyder, Stanford
Grant: U54HG006996
Download: MAZ_A549.jpg
Documents: michael-snyder:IP Protocol (Light Chain Specific Secondary) 092313
encode:TF_Antibody_Characterization_ENCODE3_May2016.pdf

Method: immunoprecipitation followed by mass spectrometry

Attachment PDF Icon

exempt from standards

Caption: IP followed by mass spectrometry: Briefly, K562 whole cell lysates were immunoprecipitated using ab85725, and the IP fraction was loaded on a 10% polyacrylamide gel (NuPAGE Bis-Tris Gel) and separated with an invitrogen NuPAGE electrophoresis system. The gel was silver-stained, gel fragments corresponding to the bands indicated were excised and destained using the SilverSNAP Stain for Mass Spectrometry (Pierce). Then proteins were treated with trypsin using the in-gel digestion method. Digested proteins were analyzed on an LTQ-Orbitrap (Thermo Scientific) by the nanoLC-ESI-MS/MS technique. Peptides were identified by the SEQUEST algorithm and filtered with a high confidence threshold (protein false discovery rate <1%, 2 peptides per protein minimum).
Submitter comment: Though not at expected size, IP-MS still identifies protein of interest enriched in immunoreactive bands
Reviewer comment: MAZ is not within the top 20 ranked by fold enrichment in band A (signal at expected size) but is for band B (not at expected size).
Submitted by: Kathrina Onate
Lab: Michael Snyder, Stanford
Grant: U54HG004558
Download: MAZ_FINAL_AIM MAZanalysis.pdf
Documents: encode:Antibody_Characterization_ENCODE3_August2015.pdf

MCF-7

Method: immunoprecipitation

compliant

Caption: Immunoprecipitation was performed on nuclear extracts from the cell line: MCF-7 using the antibody ab85725. The image shows western blot analysis of input, flowthrough, immunoprecipitate, and mock immunoprecipitate using IgG. Target molecular weight: 48.608.
Submitted by: Nathaniel Watson
Lab: Michael Snyder, Stanford
Grant: U54HG006996
Download: MAZ_MCF7.jpg
Documents: michael-snyder:IP Protocol (Light Chain Specific Secondary) 092313
encode:TF_Antibody_Characterization_ENCODE3_May2016.pdf

Method: immunoprecipitation

Attachment PDF Icon

not reviewed

Submitted by: Michael Snyder
Lab: Michael Snyder, Stanford
Grant: RC2HG005602
Download: mouse_MAZ_ab85725_validation_Snyder.pdf

Method: immunoprecipitation followed by mass spectrometry

Attachment PDF Icon

not reviewed

Submitted by: Michael Snyder
Lab: Michael Snyder, Stanford
Grant: RC2HG005602
Download: mouse_MAZ_ab85725_validation_Snyder.pdf

GM12878K562HeLa-S3HepG2

Method: immunoblot

compliant

Caption: A. Western blot using ab85724. Lanes contain nuclear lysates from GM12878 cells (lane 1), K562 cells (lane 2), HeLa-S3 cells (lane 3), and HepG2 cells (lane 4). Expected size: ~48.6kD
Reviewer comment: May be exempt from standard if IP-MS is deemed compliant.
Submitted by: Kathrina Onate
Lab: Michael Snyder, Stanford
Grant: U54HG004558
Download: WB Snyder AIM.png
Documents: encode:Antibody_Characterization_ENCODE3_August2015.pdf