H2ak119ub1

Manufactured by Cell Signaling Technology

H2AK119ub1 is a monoclonal antibody that specifically recognizes the Lys119-ubiquitinated form of histone H2A protein. It is designed for use in various applications such as Western blotting, immunoprecipitation, and immunofluorescence to detect and study the Lys119-ubiquitination of histone H2A.

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Lab products found in correlation

H3k27me3, by Cell Signaling Technology (3 mentions) Ring1b, by Cell Signaling Technology (2 mentions) Flag tag (flag), by Merck Group (1 mentions) H3k4me2, by Active Motif (1 mentions) Foxk1, by Santa Cruz Biotechnology (1 mentions) Hcfc1, by Merck Group (1 mentions) Ring1a, by Cell Signaling Technology (1 mentions) H2a z, by Cell Signaling Technology (1 mentions) H3k4me3, by Cell Signaling Technology (1 mentions) Vinculin, by Merck Group (1 mentions) Anti flag m2, by Merck Group (1 mentions) Suz12, by Cell Signaling Technology (1 mentions) Foxk1, by Abcam (1 mentions) Hcfc1, by Fortis Life Sciences (1 mentions) Micrococcal nuclease, by Roche (1 mentions) Protease inhibitor cocktail, by Roche (1 mentions) H3k9me3, by Active Motif (1 mentions) Bioruptor, by Roche (1 mentions) Simplechip enzymatic chromatin ip kit, by Cell Signaling Technology (1 mentions) Cul4b, by Merck Group (1 mentions)

Spelling variants of this product

Anti-H2AK119Ub1 (2 citations)

4 protocols using h2ak119ub1

Comprehensive Antibody Panel for Chromatin Studies

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BAP1 (1/500 dilution; C-4; sc-28383), FOXK1 (1/500 dilution; G-4; sc-373810), YY1 (1/500 dilution; sc-7341) and RAR-alpha (1/500 dilution; sc-551 × ) antibodies were purchased from Santa-Cruz; FLAG (1/1000 dilution; M2; F1804) was purchased from Sigma; HCFC1 (1/1000 dilution; A301-400A) and RNF2 (1/1000 dilution; A302-869A) antibodies were purchased from Bethyl Laboratories; Lamin B1 (1/3000 dilution; ab16048); RING1A (1/1000 dilution; 2820S), RING1B (1/1000 dilution; D22F2; 5694S) H2AK119ub1 (1/3000 dilution; D27C4; 8240S), H3K27me3 (1/3000 dilution; C36B11, 9733S), H3K4me3 (1/3000 dilution; C42D8, 9751) and H4 (1/3000 dilution; 2935S) antibodies, were purchased from Cell Signaling Technology; H2A.Z (1/1000 dilution; 39113), H2B (1/1000 dilution; 5HH2-2A8; 61037); H2BK120ub (1/1000 dilution; C56; 39623), H3 (1/3000 dilution; C-terminal; 39163), and KDM1B (1/1000 dilution; 61457) antibodies were purchased from Active Motif; H3K4me2 (1/3000 dilution; MCA-MAB10003-100-Ex) antibody was purchased from Cosmo Bio; alpha-Tubulin (1/3000 dilution; 1F4E3; A01410) was purchased from Genscript.

Campagne A., Lee M.K., Zielinski D., Michaud A., Le Corre S., Dingli F., Chen H., Shahidian L.Z., Vassilev I., Servant N., Loew D., Pasmant E., Postel-Vinay S., Wassef M, & Margueron R. (2019). BAP1 complex promotes transcription by opposing PRC1-mediated H2A ubiquitylation. Nature Communications, 10, 348.

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Generation and Characterization of Antibodies for BAP1 and ASXL1 Proteins

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Monoclonal antibodies to BAP1 (M2, available from Diagenode as C15200212) and ASXL1 (MAb32) were generated using standard protocols following immunization of BALB/c mice with the full-length BAP1 and ASXL1 human proteins, respectively. These antibodies were used in western blotting. Polyclonal mouse antisera from mice hyperimmunized by human BAP1 protein were used for ChIP. In addition, the following antibodies were used for western blotting and/or ChIP assays as indicated: FOXK1 (Abcam, ab18196), FOXK2 (Abcam, ab83286), HCFC1 (Bethyl, A301-399), H2A (Abcam, ab18255), H2AK119ub1 (Cell Signaling Technology, 8240), H3K27me3 (Cell Signaling Technology, 9733), RING1B (Cell Signaling Technology, 5694), SUZ12 (Cell Signaling Technology, 3737), anti-FLAG M2 (Merck, F1804), and Vinculin (Merck, V4505).

Kolovos P., Nishimura K., Sankar A., Sidoli S., Cloos P.A., Helin K, & Christensen J. (2020). PR-DUB maintains the expression of critical genes through FOXK1/2- and ASXL1/2/3-dependent recruitment to chromatin and H2AK119ub1 deubiquitination. Genome Research, 30(8), 1119-1130.

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Chromatin Immunoprecipitation Sequencing Protocol

Cited 2 times

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The ULI-N-ChIP-seq protocol^{65 (link)} was used to generate ChIP-seq libraries, with minor modifications. Briefly, chromatin was fragmented with 3.33 units of Micrococcal Nuclease (NEB), diluted in native ChIP buffer (20 mM Tris-HCl pH 8.0, 2 mM EDTA; 150 mM NaCl, and 0.1% Triton X-100) containing 1 mM PMSF and EDTA-free protease inhibitor cocktail (Roche) and sonicated three times with 5-second cycles on low power (Diagenode Bioruptor). Chromatin fragments were then split into two aliquots (~1000 cells/ChIP) and incubated with each of the histone methylation antibodies at 4 °C overnight. Antibodies used for ChIP experiments were H3K9me3 (39161, lot 13509002, Active Motif, 125 ng) and H2AK119ub1 (8240, lot 6, Cell Signaling, 500 ng). Following purification of ChIPed DNA by AMPure XP beads, libraries were constructed, pooled and sequenced as described above. Libraries were sequenced either on the NextSeq 500 platform with 76 paired-end reads, high-output mode (as for RNA-seq) or on the NextSeq 2000 platform with 66 paired-end reads, P2-output mode. ChIP-seq reads were aligned to the mouse genome (mm10) using bwa^{103 (link)}. PCR duplicates were removed by Picard-tools (http://broadinstitute.github.io/picard) and reads with low mapping quality (MAPQ < 5) were excluded by Samtools (http://www.htslib.org/). Processed reads were then used for calculating RPKM values by VisR^{104 (link)}.

Mochizuki K., Sharif J., Shirane K., Uranishi K., Bogutz A.B., Janssen S.M., Suzuki A., Okuda A., Koseki H, & Lorincz M.C. (2021). Repression of germline genes by PRC1.6 and SETDB1 in the early embryo precedes DNA methylation-mediated silencing. Nature Communications, 12, 7020.

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Chromatin Immunoprecipitation Protocol for Epigenetic Profiling

Cited 1 time

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ChIP was conducted using the SimpleChIP® Enzymatic Chromatin IP Kit (Cell Signaling Technology, Cat# 9003). In brief, 1 × 10⁷ cells were cross-linked with 1.5 % formaldehyde. Subsequently, nuclei were collected, and chromatin was digested, followed by overnight incubation with 1-2 μg of the respective antibody. After mixing with magnetic beads for 2 h, the mixtures were subjected to washing steps with low and high salt buffers. Subsequently, DNA was extracted from the beads and precipitated. The enrichment of the DNA was analyzed by RT-qPCR using primers specific for the target gene promoter [25 (link)]. The antibodies used for ChIP included CUL4B (Sigma-Aldrich Cat# C9995, RRID: AB_1840781), EZH2 (Cell Signaling Technology, Cat# 5246S), H2AK119ub1 (Cell Signaling Technology, Cat# 8240S) and H3K27me3 (Cell Signaling Technology, Cat# 9733S).

Guo B., Zheng Y., Fan Y., Yang Y., Wang Y., Qin L., An Y., Xu X., Zhang X., Sun G., Dou H., Shao C., Gong Y., Jiang B, & Hu H. (2024). Enhanced ApcMin/+ adenoma formation after epithelial CUL4B deletion by recruitment of myeloid-derived suppressor cells. Neoplasia (New York, N.Y.), 53, 101005.

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