Proteomics

Dataset Information

0

Lysine fatty-acyl H3 peptide pulldown with HeLa SILAC nuclear extract


ABSTRACT: Histone H3 peptides with acyl modification on either K9 or K27 were used for peptide pull-down with stable isotope (light: K0R0, heavy: K8R10) labeled Hela nuclear extract. The acyl modifications are: acetyl (Ac), propionyl (Pro), Butanoyl (But), crotonyl (Cr), 3-hydroxy butanoyl (bHB), succinyl (Su), Pentanoyl (Vl), Hexanoyl (Xho) and Myristoyl (Myr). Each modified peptide is compared with an unmodified peptide with the same amino acid sequence. Both forward (unmodified-light, acyl-heavy) and reverse (unmodified-heavy, acyl-light) labeling and pull-down experiments were performed.

INSTRUMENT(S): LTQ Orbitrap Elite

ORGANISM(S): Homo Sapiens (human)

TISSUE(S): Permanent Cell Line Cell, Cell Culture

SUBMITTER: John Coan  

LAB HEAD: Katrin Chua

PROVIDER: PXD015233 | Pride | 2019-10-02

REPOSITORIES: Pride

Dataset's files

Source:
Action DRS
H3K27Myr-fwd.raw Raw
H3K27Myr-rev.raw Raw
H3K27Vl-fwd.raw Raw
H3K27Vl-rev.raw Raw
H3K27Xho-fwd.raw Raw
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Publications

Binding to medium and long chain fatty acyls is a common property of HEAT and ARM repeat modules.

Li Tie-Mei TM   Coan John P JP   Krajewski Krzysztof K   Zhang Lichao L   Elias Joshua E JE   Strahl Brian D BD   Gozani Or O   Chua Katrin F KF  

Scientific reports 20191002 1


Covalent post-translational modification (PTM) of proteins with acyl groups of various carbon chain-lengths regulates diverse biological processes ranging from chromatin dynamics to subcellular localization. While the YEATS domain has been found to be a prominent reader of acetylation and other short acyl modifications, whether additional acyl-lysine reader domains exist, particularly for longer carbon chains, is unclear. Here, we employed a quantitative proteomic approach using various modified  ...[more]

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