ChIP-qPCR Assay for Chromatin Immunoprecipitation

ChIP‐qPCR was performed as described in Poli et al (2016 (link)) using anti‐HA probe F‐7 (Santa Cruz, sc‐7392) and anti‐Rpb1‐CTD 8WG16 (Abcam, ab817) coupled to Dynabeads (Invitrogen, protein A and sheep anti‐mouse M280 IgG). For quantitative PCR, background controls were determined using uncoupled Dynabeads and enrichment was normalized to chromatin Input. Primers used for ChIP‐qPCR are listed in Table EV2.

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Hurst V., Challa K., Jonas F., Forey R., Sack R., Seebacher J., Schmid C.D., Barkai N., Shimada K., Gasser S.M, & Poli J. (2021). A regulatory phosphorylation site on Mec1 controls chromatin occupancy of RNA polymerases during replication stress. The EMBO Journal, 40(21), e108439.

Publication 2021

anti‐HA probe F‐7 anti‐Rpb1‐CTD 8WG16 Dynabeads

Anti igg Chip Chromatin Mouse Poli Primers Protein a Sheep

Corresponding Organization :

Other organizations : Friedrich Miescher Institute, University of Basel, Weizmann Institute of Science, Institut de Génétique Humaine, University of Augsburg

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Variable analysis

independent variables

Anti-HA probe F-7 (Santa Cruz, sc-7392)
Anti-Rpb1-CTD 8WG16 (Abcam, ab817)

dependent variables

Enrichment normalized to chromatin Input

control variables

Uncoupled Dynabeads

controls

Positive control: Dynabeads coupled to anti-HA probe F-7 (Santa Cruz, sc-7392) and anti-Rpb1-CTD 8WG16 (Abcam, ab817)
Negative control: Uncoupled Dynabeads

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