recombination center
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Author(s):  
Tomohiko Hara ◽  
Taichi Tanaka ◽  
Kazuhito Nakagawa ◽  
Yuki Isogai ◽  
Takefumi Kamioka ◽  
...  

2020 ◽  
Author(s):  
Hai-Qiang Dai ◽  
Hongli Hu ◽  
Jiangman Lou ◽  
Adam Yongxin Ye ◽  
Aimee M. Chapdelaine-Williams ◽  
...  

AbstractImmunoglobulin heavy chain locus (Igh) VH, D, and JH gene segments are developmentally assembled into V(D)J exons. RAG endonuclease initiates V(D)J recombination by binding a JH-recombination signal sequence (RSS) within a chromatin-based recombination center (RC) and then, in an orientation-dependent process, scans upstream D-containing chromatin presented by cohesin-mediated loop extrusion for convergent D-RSSs to initiate DJH-RC formation1,2. In primary pro-B cells, 100s of upstream VH-associated RSSs, embedded in convergent orientation to the DJH-RC-RSS, gain proximity to the DJH-RC for VH-to-DJH joining via a mechanistically-undefined VH-locus contraction process3-7. Here, we report that a 2.4 mega-base VH locus inversion in primary pro-B cells nearly abrogates rearrangements of normally convergent VH-RSSs and cryptic RSSs, even though locus contraction per se is maintained. Moreover, this inversion activated rearrangement of both cryptic VH-locus RSSs normally in the opposite orientation and, unexpectedly, of normally-oriented cryptic RSSs within multiple, sequential upstream convergent-CBE domains. Primary pro-B cells had significantly reduced transcription of Wapl8, a cohesin-unloading factor, versus levels in v-Abl pro-B lines that lack marked locus contraction or distal VH rearrangements2,9-11. Correspondingly, Wapl depletion in v-Abl lines activated VH-locus contraction and orientation-specific RAG-scanning across the VH-locus. Our findings indicate that locus contraction and physiological VH-to-DJH joining both are regulated via circumvention of CBE scanning impediments.


2020 ◽  
Author(s):  
Zhaoqing Ba ◽  
Jiangman Lou ◽  
Edward W. Dring ◽  
Adam Yongxin Ye ◽  
Sherry G. Lin ◽  
...  

AbstractRAG endonuclease initiates V(D)J recombination in progenitor (pro)-B cells1. Upon binding a recombination center (RC)-based JH, RAG scans upstream chromatin via loop extrusion, potentially mediated by cohesin2–10, to locate Ds and assemble a DJH-based RC11. CTCF looping factor-bound elements (CBEs) within IGCR1 upstream of Ds impede RAG-scanning12–15; but their inactivation allows scanning to proximal VHs where additional CBEs activate rearrangement and impede scanning any further upstream15, 16. Distal VH utilization is thought to involve diffusional RC access following large-scale Igh locus contraction17–23. Here, we test the potential of linear RAG-scanning to mediate distal VH usage in G1-arrested, v-Abl-pro-B cell lines24, 25, which undergo robust D-to-JH but little VH-to-DJH rearrangements, presumably due to lack of locus contraction11, 15. Through an auxin-inducible approach26, 27, we degrade the cohesin-component Rad214, 7, 27 or CTCF7, 9 in these G1-arrested lines, which maintain substantial viability throughout four-day experiments. Rad21 degradation eliminated all V(D)J recombination and RAG-scanning-associated interactions, except RC-located DQ52-to-JH joining in which synapsis occurs by diffusion11. Remarkably, while CTCF degradation suppressed most CBE-based chromatin interactions, it promoted robust RC interactions with, and robust VH-to-DJH joining of, distal VHs, with patterns similar to those of “locus-contracted” primary pro-B cells. Thus, down-modulation of CTCF-bound scanning-impediment activity promotes cohesin-driven RAG-scanning across the 2.7Mb Igh locus.


2020 ◽  
Vol 8 (26) ◽  
pp. 12964-12967
Author(s):  
Xie Zhang ◽  
Jimmy-Xuan Shen ◽  
Mark E. Turiansky ◽  
Chris G. Van de Walle

BiPb is not a recombination center in hybrid perovskites, but promotes the formation of the actual recombination centers—iodine interstitials.


2019 ◽  
Vol 21 (3) ◽  
pp. 1491-1496 ◽  
Author(s):  
Constantin A. Walenta ◽  
Sebastian L. Kollmannsberger ◽  
Carla Courtois ◽  
Rui N. Pereira ◽  
Martin Stutzmann ◽  
...  

The photocatalytic H2 evolution on co-catalyst loaded titania is interpreted by a new mechanism, in which the co-catalyst acts as a recombination center for hydrogen and not as a reduction site of a photoreaction.


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