2007
DOI: 10.1073/pnas.0710179104
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Protein characterization of Saccharomyces cerevisiae RNA polymerase II after in vivo cross-linking

Abstract: To characterize proteins associated with active transcription complexes, we purified RNA polymerase II (pol II) from Saccharomyces cerevisiae after fixing live cells with formaldehyde. The approach mimics ChIP and requires solubilizing cross-linked complexes with sonication. Pol II was affinity-purified, and associated proteins were identified by MS. Several classes of proteins depended on cross-linking, including Mediator, general transcription factors, elongation factors, ribonucleoprotein particle (RNP) pro… Show more

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Cited by 57 publications
(50 citation statements)
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“…This result reaffirms that the QTAX strategy is effective in capturing both stable and/or weak/transient protein interactions. A similar observation was reported for RNA polymerase II-interacting proteins when a similar strategy was applied for capturing its interactors by in vivo formaldehyde cross-linking and TAP (18).…”
Section: Purification and Identification Of Pips By Qtax-based Tag-tementioning
confidence: 57%
“…This result reaffirms that the QTAX strategy is effective in capturing both stable and/or weak/transient protein interactions. A similar observation was reported for RNA polymerase II-interacting proteins when a similar strategy was applied for capturing its interactors by in vivo formaldehyde cross-linking and TAP (18).…”
Section: Purification and Identification Of Pips By Qtax-based Tag-tementioning
confidence: 57%
“…The interactions of the S. cerevisiae protein Npl3, with Air2, Ded1, Gbp2, Snp1, and Yra1 were reported in large-scale studies elsewhere, detected by AP-MS and/or yeast two-hybrid techniques (16,(27)(28)(29). As such, it was important for these to be first verified in the bacterial C2H system before the effect of arginine methylation was examined.…”
Section: Verification Of the Interactions Of Npl3-mentioning
confidence: 99%
“…To circumvent these problems, in vivo chemical crosslinking has been successfully employed to stabilize protein interactions in native cells or tissues prior to cell lysis (10 -16). The resulting covalent bonds formed between interacting partners allow affinity purification under stringent and fully denaturing conditions, consequently reducing nonspecific background while preserving stable and weak/transient interactions (12)(13)(14)(15)(16). Subsequent mass spectrometric analysis can reveal not only the identities of interacting proteins, but also cross-linked amino acid residues.…”
mentioning
confidence: 99%