Anti-BMAL1 antibody
5
(7 Reviews)
|
(103 Publications)
Anti-BMAL1 antibody (ab93806) is a rabbit polyclonal antibody detecting BMAL1 in Western Blot, IP. Suitable for Human, Mouse.
- Over 80 publications
- Trusted since 2010
View Alternative Names
ARNTL, BHLHE5, MOP3, PASD3, BMAL1, Basic helix-loop-helix ARNT-like protein 1, Aryl hydrocarbon receptor nuclear translocator-like protein 1, Basic-helix-loop-helix-PAS protein MOP3, Brain and muscle ARNT-like 1, Class E basic helix-loop-helix protein 5, Member of PAS protein 3, PAS domain-containing protein 3, bHLH-PAS protein JAP3, bHLHe5
- WB
Unknown
Western blot - Anti-BMAL1 antibody (AB93806)
All lanes:
Western blot - Anti-BMAL1 antibody (ab93806) at 1/2000 dilution
Lane 1:
HeLa lysate at 50 µg
Lane 2:
HeLa lysate at 15 µg
Lane 3:
HeLa lysate at 5 µg
Lane 4:
293T at 50 µg
Lane 5:
NIH3T3 at 50 µg
Predicted band size: 68 kDa
true
Exposure time: 3min
- IP
Unknown
Immunoprecipitation - Anti-BMAL1 antibody (AB93806)
ab93806 at 1 µg/ml detecting BMAL1 in HeLa whole cell lysate by WB following IP.
Lane 1 : IP with an antibody which recognizes an upstream epitope of BMAL1
Lane 2 : ab93806 at 3µg/mg of lysate
Lane 3 : control IgG.
In each case, 1 mg of lysate was used for IP and 20% of the IP was loaded.
Detection : Chemiluminescence an with exposure time of 30 seconds
All lanes:
1 mg of lysate was used for IP and 20% of the IP was loaded
Lane 1:
<a href='/en-us/products/unavailable/kat13d-clock-antibody-ab93805'>ab93805</a> at 3µg/mg of lysate
Lane 2:
IP with an antibody which recognizes an downstream epitope of KAT13D/CLOCK
Lane 3:
control IgG.
Predicted band size: 68 kDa
false
- WB
CiteAb
Western blot - Anti-BMAL1 antibody (AB93806)
Western Blotting using Anti-BMAL1 antibody, ab93806. Publication image from Armirotti, A. et al., 2017, Nat Commun, 28186121. Legend direct from paper.
Altered VIP expression in the SCN and impaired cortical and hippocampal oscillations in Bmal1cKO mice.(a) Representative micrographs of VIP immunostaining in the SCN of Bmal1cKO and control mice in 12 : 12 h LD cycles at ZT12. Quantification of fluorescence intensity demonstrates higher VIP levels in Bmal1cKO at ZT12 compared with control animals (paired t-test *P<0.05 versus ZT0 and #P<0.05 versus control animals). The value express the mean±s.e.m. (n=3 animals per group). Scale bar, 40 µm. (b) Analysis of Bmal1 and Per2 in the cortex (upper panels) and hippocampus (lower panels) of control (blue) and Bmal1cKO (red) mice, showing impaired rhythmic expression in mutant mice. Experimental data were cosine fitted. Samples were collected from mice under 12 : 12 h LD cycles. It is noteworthy that the ZT24 time point is the ZT0 time point, shown again. Means±s.e.m. of five animals per group at each time point (paired t-test; *P<0.05, **P<0.01 and ***P<0.001 versus control animals). (c) Representative images of cortical BMAL1 and PER2 western blottings, showing no oscillation of those proteins in Bmal1cKO as compared ith control mice (n=3 animals per group and time point).
false
- WB
CiteAb
Western blot - Anti-BMAL1 antibody (AB93806)
Western Blotting using Anti-BMAL1 antibody, ab93806. Publication image from Armirotti, A. et al., 2017, Nat Commun, 28186121. Legend direct from paper.
Bmal1 knockdown in astrocytes suppresses entrainment of co-cultured cortical neurons in vitro.(a) Primary cortical astrocytes were transfected with scramble (Scrbl) or Bmal1 siRNAs. After 48 h, astrocytes were synchronized with 100 nM of Dexamethasone for 2 h (Astro Dexa). After washing, astrocytes were placed in co-culture with asynchronous cortical neurons without physical contact, but sharing the same culture media. (b) Bmal1, Cry1, Per2 and BMAL1 target Dbp were analysed in astrocytes (upper panels) and neurons (lower panels) at the indicated time points by quantitative PCR. Graphs show the mean±s.e.m. of the cosine-fitted curves from three experiments performed in triplicate. (c) Representative images of western blottings for BMAL1 in primary astrocytes (left panels) or CRY1 in co-cultured neurons (right panels), showing expression of BMAL1 in Dexamethasone-treated astrocytes in isolated cultures (top) or Dexamethasone-treated astrocytes in co-culture with asynchronous neurons (middle and bottom), on transfection with scramble siRNAs (CSA Scrbl) or on transfection with Bmal1 siRNAs (CSA KD); (right panels) entrainment of CRY1 in cortical neurons after co-culture with Scrbl transfected synchronous astrocytes (Neu-CSA Scrbl) is not observed when co-culture is performed with arrhythmic astrocytes (Neu-CSA KD) (n=2 independent experiments).
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Reactivity data
Product details
Anti-BMAL1 antibody (ab93806) is a rabbit polyclonal antibody and is validated for use in Western Blot (WB), Immunoprecipitation (IP) in Human, Mouse samples.
What is the molecular weight of BMAL1?
Anti-BMAL1 (ab93806) specifically detects a band for BMAL1 (UniProt: O00327) at a molecular weight of 69kDa.
Trusted by the scientific community
Anti-BMAL1 (ab93806) was first used in a scientific publication in 2010 and has been cited over 80 times in peer-reviewed journals.
Reviewed by scientists
Anti-BMAL1 (ab93806) has over 5 independent reviews from customers.
Properties and storage information
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Purification notes
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Appropriate long-term storage conditions
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Target data
Publications (103)
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Molecular metabolism 101:102249 PubMed40947011
2025
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iScience 28:112786 PubMed40585367
2025
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Nature chemical biology 21:736-745 PubMed40133642
2025
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European journal of medical research 30:29 PubMed39810231
2025
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The EMBO journal 43:6052-6075 PubMed39433902
2024
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International journal of molecular sciences 25: PubMed39408733
2024
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Science advances 10:eado1458 PubMed39331712
2024
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ERJ open research 10: PubMed39010889
2024
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Cell reports 43:114380 PubMed38935503
2024
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The Journal of biological chemistry 300:107434 PubMed38830405
2024
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Product promise
Please note: All products are 'FOR RESEARCH USE ONLY. NOT FOR USE IN DIAGNOSTIC OR THERAPEUTIC PROCEDURES'.
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