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Anti aurora b

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Anti-Aurora B is a lab equipment product that functions as an inhibitor of the Aurora B kinase. It is used in research applications to study the role of the Aurora B kinase in cellular processes.

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Lab products found in correlation

Anti phospho histone h3 ser10, by Merck Group (3 mentions) Alexa fluor 488 or 555, by Thermo Fisher Scientific (2 mentions) Sc 47739, by Merck Group (2 mentions) Anti phospho histone gamma h2ax, by Merck Group (2 mentions) Ab62623, by Abcam (2 mentions) Antifade mounting medium, by Vector Laboratories (2 mentions) Ab68167, by Abcam (2 mentions) Epitope retrieval solution, by IHC World (2 mentions) Anti β actin, by Merck Group (2 mentions) Ab64548, by Abcam (1 mentions) Alexa fluor 488, by Thermo Fisher Scientific (1 mentions) Anti bromodeoxyuridine, by Roche (1 mentions) Anti sarcomeric alpha actinin, by Abcam (1 mentions) Peroxidase conjugated secondary antibody, by Jackson ImmunoResearch (1 mentions) Anti ha, by Merck Group (1 mentions) Ecl detection system, by Cytiva (1 mentions) Anti flag m2, by Merck Group (1 mentions) Multi gauge, by Fujifilm (1 mentions) Las 4000, by Cytiva (1 mentions) Protein assay, by Bio-Rad (1 mentions)

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Aurora B (5 citations)

5 protocols using anti aurora b

1

Immunohistochemistry of Cardiac Tissues

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Tissues were fixed in 4% paraformaldehyde in PBS overnight at 4°C
and incubated in 30% sucrose in PBS at 4°C overnight. Tissues were
embedded in tissue freezing medium and cut 8 μm thicknesses. For antigen
retrieval, either 1 mM EDTA with 0.05% Tween 20 in boiling water or epitope
retrieval solution (IHC World) in a steamer (IHC-Tek Epitope Retrieval Streamer
Set) were used, then sections were blocked with 10% serum from the host animal
of secondary antibodies, and incubated with primary anti-bodies overnight at 4
°C. The sections were subsequently washed with PBS and incubated with
corresponding secondary antibodies conjugated to Alexa Fluor 488 or 555
(Invitrogen). The slides were mounted in antifade mounting medium (Vector
Laboratories, Burlingame, California). Primary antibodies used are as follows:
anti-phospho histone H3 Ser10 (Millipore 06–570, 1:100), anti-aurora B
(Sigma A5102, 1:100), anti-troponin T, cardiac isoform Ab-1, clone 13–11
(Thermo Scientific MS-295-P1, 1:100), anti-sarcomeric α-actinin (Abcam,
ab68167, 1:100), anti-8 hydroxyguanosine (Abcam ab62623, 1:50),
anti-phosphorylated ATM (Santa Cruz Biotechnology sc-47739, 1:100),
Anti-phospho-Histone gamma H2AX (Millipore-Sigma 05–636). DAPI was used
for the nuclear staining.
Cardoso A.C., Lam N.T., Savla J.J., Nakada Y., Pereira A.H., Elnwasany A., Menendez-Montes I., Ensley E.L., Petric U.B., Sharma G., Sherry A.D., Malloy C.R., Khemtong C., Kinter M.T., Tan W.L., Anene-Nzelu C.G., Foo R.S., Nguyen N.U., Li S., Ahmed M.S., Elhelaly W.M., Abdisalaam S., Asaithamby A., Xing C., Kanchwala M., Vale G., Eckert K.M., Mitsche M.A., McDonald J.G., Hill J.A., Huang L., Shaul P.W., Szweda L.I, & Sadek H.A. (2020). Mitochondrial Substrate Utilization Regulates Cardiomyocyte Cell Cycle Progression. Nature metabolism, 2(2), 167-178.
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2

Immunohistochemistry of Cardiac Tissues

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Tissues were fixed in 4% paraformaldehyde in PBS overnight at 4°C
and incubated in 30% sucrose in PBS at 4°C overnight. Tissues were
embedded in tissue freezing medium and cut 8 μm thicknesses. For antigen
retrieval, either 1 mM EDTA with 0.05% Tween 20 in boiling water or epitope
retrieval solution (IHC World) in a steamer (IHC-Tek Epitope Retrieval Streamer
Set) were used, then sections were blocked with 10% serum from the host animal
of secondary antibodies, and incubated with primary anti-bodies overnight at 4
°C. The sections were subsequently washed with PBS and incubated with
corresponding secondary antibodies conjugated to Alexa Fluor 488 or 555
(Invitrogen). The slides were mounted in antifade mounting medium (Vector
Laboratories, Burlingame, California). Primary antibodies used are as follows:
anti-phospho histone H3 Ser10 (Millipore 06–570, 1:100), anti-aurora B
(Sigma A5102, 1:100), anti-troponin T, cardiac isoform Ab-1, clone 13–11
(Thermo Scientific MS-295-P1, 1:100), anti-sarcomeric α-actinin (Abcam,
ab68167, 1:100), anti-8 hydroxyguanosine (Abcam ab62623, 1:50),
anti-phosphorylated ATM (Santa Cruz Biotechnology sc-47739, 1:100),
Anti-phospho-Histone gamma H2AX (Millipore-Sigma 05–636). DAPI was used
for the nuclear staining.
Cardoso A.C., Lam N.T., Savla J.J., Nakada Y., Pereira A.H., Elnwasany A., Menendez-Montes I., Ensley E.L., Petric U.B., Sharma G., Sherry A.D., Malloy C.R., Khemtong C., Kinter M.T., Tan W.L., Anene-Nzelu C.G., Foo R.S., Nguyen N.U., Li S., Ahmed M.S., Elhelaly W.M., Abdisalaam S., Asaithamby A., Xing C., Kanchwala M., Vale G., Eckert K.M., Mitsche M.A., McDonald J.G., Hill J.A., Huang L., Shaul P.W., Szweda L.I, & Sadek H.A. (2020). Mitochondrial Substrate Utilization Regulates Cardiomyocyte Cell Cycle Progression. Nature metabolism, 2(2), 167-178.
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3

Multiparametric Immunohistochemistry: Cellular Analysis

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Following antigen retrieval with 1mM EDTA in boiling water, sections were blocked with 10% serum from host animal of secondary antibodies, and incubated with primary antibodies overnight at 4°C. Sections were subsequently washed with PBS and incubated with corresponding secondary antibodies conjugated to Alexa Fluor 350, 488 or 555 (Invitrogen). Primary antibodies used are following: anti-phospho Histone H3 Ser10 (Millipore #06–570, 1:100), anti-Aurora B (Sigma A5102, 1:100), anti-Troponin T, Cardiac Isoform Ab-1, Clone 13–11 (Thermo scientific MS-295-P1, 1:100), anti-Bromodeoxyuridine (Roche #11170376001, 1:25), anti-Sarcomeric Alpha Actinin (Abcam, ab68167, 1:100), anti-oxoguanine 8 (Abcam Ab64548, 1:100), anti-phosphorilated ATM (Santa Cruz Biotechnology sc-47739, 1:100), anti-Wee1 (Abcam ab137377, 1:100). Anti-weat germ agglutinin (WGA) conjugated to Alexa Fluor 488 (50 µg/ml, Invitrogen).
Puente B.N., Kimura W., Muralidhar S.A., Moon J., Amatruda J.F., Phelps K.L., Grinsfelder D., Rothermel B.A., Chen R., Garcia J.A., Santos C.X., Thet S., Mori E., Kinter M.T., Rindler P.M., Zacchigna S., Mukherjee S., Chen D.J., Mahmoud A.I., Giacca M., Rabinovitch P.S., Aroumougame A., Shah A.M., Szweda L.I, & Sadek H.A. (2014). The Oxygen Rich Postnatal Environment Induces Cardiomyocyte Cell Cycle Arrest Through DNA Damage Response. Cell, 157(3), 565-579.
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4

Immunoblotting and IP Experiments Protocol

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Immunoblotting and IP experiments were performed as described before19 (link). Nocodazole was used at 100 ng/ml for 16 hours. The following primary antibodies were used for immunoblotting: anti-Ataxin-10, anti-Aurora B, anti-β-actin, anti-HA and anti-FLAG M2 (Sigma). Peroxidase-conjugated secondary antibodies were from JacksonImmuno Research. Blotted proteins were visualized using the ECL detection system (Amersham). Signals were detected by a LAS-4000, and analyzed using Multi Gauge (Fujifilm).
Tian J., Tian C., Ding Y., Li Z., Geng Q., Xiahou Z., Wang J., Hou W., Liao J., Dong M.Q., Xu X, & Li J. (2015). Aurora B-dependent phosphorylation of Ataxin-10 promotes the interaction between Ataxin-10 and Plk1 in cytokinesis. Scientific Reports, 5, 8360.
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5

Immunoblotting Analysis of Cell Signaling

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Cells were cultured for 2.5 h without (w.o.) or in the presence of inhibitor at the indicated concentrations. After cell lysis, sonification, and measuring of the protein concentration using BioRad Protein Assay (Biorad, Munich, Germany), protein extracts were electrophoretically separated on SDS-PAGE gels and immunoblotted with indicated antibodies. Anti-Aurora A, anti-Aurora B, Anti- pHistone-3 (Serine 10), and anti-β-Actin antibodies were obtained from Sigma-Aldrich (Heidelberg, Germany), Anti-Flag (M2) antibody from Stratagene (Heidelberg, Germany). Anti-Abl antibody (8E9) was purchased from BD Biosciences (San Jose, CA), anti-STAT5 antibody (C-17) from Santa Cruz Biotechnology Inc. (Heidelberg, Germany). Detection of phosphotyrosine was performed using a mixture of the antibodys 4G10 (Millipore, Schwalbach, Germany) and PY20 (BD Biosciences, San Jose, CA). pSTAT5 antibody was a kind gift from T. Wheeler (Hamilton, New Zealand; Wheeler et al., 2001). Bands were visualized using SuperSignal Chemoluminescence substrate (Pierce, Rockford, USA).
Illert A.L., Seitz A.K., Rummelt C., Kreutmair S., Engh R.A., Goodstal S., Peschel C., Duyster J, & von Bubnoff N. (2014). Inhibition of Aurora Kinase B Is Important for Biologic Activity of the Dual Inhibitors of BCR-ABL and Aurora Kinases R763/AS703569 and PHA-739358 in BCR-ABL Transformed Cells. PLoS ONE, 9(11), e112318.
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