Proteomics

Dataset Information

0

D6_T3


ABSTRACT: To examine the signaling pathways active downstream ACKR2, both in constitutive and ligand-stimulated conditions, we carried out a large-scale mass spec-based quantitative phosphoproteomic analysis by SILAC technique. ACKR2 has been expressed in HEK293T cells using a tetracycline-inducible system and stimulated with the common ligand CCL3L1. Using computational approaches, we performed a comparative system-based analysis of the ACKR2- and CCR5-mediated phosphoproteomes.

INSTRUMENT(S): LTQ Orbitrap Velos

ORGANISM(S): Homo Sapiens (human)

SUBMITTER: gabriella tedeschi  

LAB HEAD: Gabriella Tedeschi

PROVIDER: PXD009835 | Pride | 2023-03-10

REPOSITORIES: Pride

Dataset's files

Source:
Action DRS
EluatoF_1_T3.raw Raw
EluatoF_2_T3.raw Raw
EluatoF_3_T3.raw Raw
EluatoG_1_T3.raw Raw
EluatoG_2_T3.raw Raw
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Publications


ACKR2 is an atypical chemokine receptor which is structurally uncoupled from G proteins and is unable to activate signaling pathways used by conventional chemokine receptors to promote cell migration. Nonetheless, ACKR2 regulates inflammatory and immune responses by shaping chemokine gradients in tissues <i>via</i> scavenging inflammatory chemokines. To investigate the signaling pathways downstream to ACKR2, a quantitative SILAC-based phosphoproteomic analysis coupled with a systems biology appr  ...[more]

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