Gopal Karemore scite author profile

A fascinating conundrum in cell signaling is how stimulation of the same receptor tyrosine kinase with distinct ligands generates specific outcomes. To decipher the functional selectivity of EGF and TGF-α, which induce epidermal growth factor receptor (EGFR) degradation and recycling, respectively, we devised an integrated multilayered proteomics approach (IMPA). We analyzed dynamic changes in the receptor interactome, ubiquitinome, phosphoproteome, and late proteome in response to both ligands in human cells by quantitative MS and identified 67 proteins regulated at multiple levels. We identified RAB7 phosphorylation and RCP recruitment to EGFR as switches for EGF and TGF-α outputs, controlling receptor trafficking, signaling duration, proliferation, and migration. By manipulating RCP levels or phosphorylation of RAB7 in EGFR-positive cancer cells, we were able to switch a TGF-α-mediated response to an EGF-like response or vice versa as EGFR trafficking was rerouted. We propose IMPA as an approach to uncover fine-tuned regulatory mechanisms in cell signaling.

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Breast milk alkylglycerols sustain beige adipocytes through adipose tissue macrophages

Yu¹,

Dilbaz²,

Coßmann³

et al. 2019

164

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Stabilization of chromatin topology safeguards genome integrity

Ochs

Karemore

Miron

et al. 2019

Nature

153

119

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To safeguard genome integrity in response to DNA double-strand breaks (DSB), mammalian cells mobilize the neighboring chromatin to shield DNA ends against excessive resection that could undermine repair fidelity and cause damage to healthy chromosomes 1. This form of genome surveillance is orchestrated by 53BP1, whose accumulation at DSBs triggers sequential recruitment of RIF1 and the shieldin-CST-Polα complex 2. How this pathway reflects and impacts on the three-dimensional (3D) nuclear architecture is not known. Here, we applied super-resolution microscopy to show that 53BP1 and RIF1 form an autonomous functional module that stabilizes 3D chromatin topology at sites of DNA breakage. This is initiated by 53BP1 accrual at compact chromatin regions colocalizing with topology-associated domain (TAD) sequences and followed by RIF1 recruitment to boundaries between such domains. The alternating 53BP1 and RIF1 distribution stabilizes several neighboring TAD-sized structures at a single DBS site to an ordered, circular arrangement. Depletion of 53BP1 or RIF1 (but not shieldin) disrupts this arrangement, leading to decompaction of DSBflanking chromatin, reduction of interchromatin space, aberrant spreading of DNA repair proteins, and DNA-end hyper-resection. Similar topological distortions are triggered by depletion of cohesin, suggesting that maintenance of chromatin structure after DNA breakage involves basic mechanisms that shape 3D nuclear organization. Since topological stabilization of DSB-flanking chromatin is independent of DNA repair, we propose that besides providing a structural scaffold to protect DNA ends against aberrant processing, 53BP1 and RIF1 safeguard epigenetic integrity at loci disrupted by DNA breakage. quantitative nanoscopy texture (QUANTEX) analysis tool, which indeed revealed a significant increase in 53BP1-MD Mean breadth and Principal axis length (Fig. 1e, f; Extended Data Fig. 3a-c). It was further reproduced by silencing RIF1 with multiple siRNAs, by replacing endogenous 53BP1 with a mutant unable to promote RIF1 recruitment 10 , and in several cancer-derived as well as non-cancerous cells (Extended Data Fig. 4a-e). Together, these data indicate that 53BP1 and RIF1 form an autonomous module where RIF1 is required to stabilize 53BP1-NDs into ordered, circular chromatin architecture (Extended Data Fig. 4f). In support of this, knockdown of 53BP1 or RIF1 phenocopied each other by disrupting γH2AX-marked chromatin into disordered and elongated shapes (Extended Data Fig. 4g-i). To study how 53BP1 and RIF1 cooperate to stabilize chromatin topology, we set out to determine RIF localization with respect to 53BP1. While conventional microscopy only generally indicates 53BP1 and RIF1 proximity at DSB-sites, 3D-SIM and STED revealed that RIF1 localized to the chromatin boundaries between neighboring 53BP1-NDs (Fig. 2a). To understand the purpose of this alternating localization, we tracked 53BP1 dynamics from pre-to post-damaged state using live-cell 3D-SIM (live-SIM; Extended Data Fig. 5a). The fir...

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Gopal Karemore

Multilayered proteomics reveals molecular switches dictating ligand-dependent EGFR trafficking

Breast milk alkylglycerols sustain beige adipocytes through adipose tissue macrophages

Stabilization of chromatin topology safeguards genome integrity

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