ENCAB219NWE
Antibody against Homo sapiens ATM
Homo sapiens
HepG2
characterized to standards
- Status
- released
- Source (vendor)
- Bethyl Labs
- Product ID
- A300-135A
- Lot ID
- 1
- Characterized targets
- ATM (Homo sapiens)
- Host
- goat
- Clonality
- polyclonal
- Purification
- affinity
- Aliases
- michael-snyder:AS-856
- External resources
Characterizations
ATM (Homo sapiens)
compliant
- Caption
- IP followed by mass spectrometry. Briefly, protein was immunoprecipitated from HepG2 nuclear cell lysates using the antibody A300-135A, and the IP fraction was loaded on a 10% polyacrylamide gel (NuPAGEBis-Tris Gel) and separated with an Invitrogen NuPAGE electrophoresis system. The gel was stained by ColloidialCoomassie G-250 stain, gel fragments corresponding to the bands indicated were excised. Then proteins were trypsinized using the in-gel digestion method. Digested proteins were analyzed on an Orbitrap Elite mass spectrometer (Thermo Scientific) by the nanoLC-ESI-MS/MS technique. Peptides were identified by the SEQUEST algorithm and filtered with a high confidence threshold (Peptide false discovery rate < 1%, 2 unique peptides per protein minimum, mass error < 10 ppm).
- Submitted by
- Nathaniel Watson
- Lab
- Michael Snyder, Stanford
- Grant
- U54HG006996
- Download
- ATM_A300-135A final.pdf
ATM (Homo sapiens)
HepG2
exempt from standards
- Caption
- Immunoprecipitation was performed on nuclear extracts from the cell line: HepG2, using the antibody A300-135A. The blot shows western blot analysis of input, flowthrough, immunoprecipitate and mock immunoprecipitate using IgG.
- Submitter comment
- Sorry, we didn't have a better ladder.
- Reviewer comment
- Band is very small, is there a bigger ladder that can be used? It's tough evaluate whether it's within 20% of expected size.
- Submitted by
- Denis Salins
- Lab
- Michael Snyder, Stanford
- Grant
- U54HG006996
ATM (Homo sapiens)
HepG2
compliant
- Caption
- Immunoprecipitation was performed on nuclear extracts from the cell line HepG2 using the antibody A300-135A. Lane 1: input nuclear lysate. Lane 2: material immunoprecipitated with antibody. Lane 3: material immunoprecipitated using control IgG. Marked bands were excised from gel and subjected to analysis by mass spectrometry. Target molecular weight: 350.714.
- Submitted by
- Nathaniel Watson
- Lab
- Michael Snyder, Stanford
- Grant
- U54HG006996
- Download
- MS1045_1_ATM-A300-135A.JPG