Phosphorylation of the synaptonemal complex protein SYP-1 promotes meiotic chromosome segregation

Sato-Carlton, Aya; Tabuchi, Chihiro; Chartrand, Stephane Kazuki; Uchino, Tomoki; Carlton, Peter M.

doi:10.1101/211672

Cited by 12 publications

(27 citation statements)

References 69 publications

(99 reference statements)

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“…To understand regulation of meiotic proteins by post-translational modification, we previously carried out mass spectrometry to identify phosphorylated proteins in C. elegans adult hermaphrodites [16] . In two independent experiments, we found that the chromosome axis protein HIM-3 is phosphorylated at its C-terminus.…”

Section: Him-3 Hormad1/2 Is Phosphorylated At the Conserved Closure Mmentioning

confidence: 99%

“…As oocyte precursor cells progress into late pachytene, designate crossovers, and begin to differentiate long and short arms, HIM-3phos antibody staining becomes enriched on only a small, terminal part of the SC, in contrast to panHIM-3 staining which remains on the full length of the SC, suggesting that phosphorylated HIM-3 becomes enriched on the short arm ( Figure 2B ). Simultaneous staining with the short arm marker SYP-1phos antibody [16] as well as the crossover designation marker COSA-1 [32] revealed that phosphorylated HIM-3 becomes enriched at short arms once crossovers are designated ( Figure 2C ). Although Ser282 is in an ATM/ATR kinase consensus site (SQ), we found that phosphorylation of HIM-3 Ser282 does not depend on these DNA damage-responsive kinases ( Supplemental Figure 1C ).…”

Section: Phosphorylated Him-3 Localizes To the Entire Length Of The Smentioning

confidence: 99%

“…The E3 ligases ZHP-1 and ZHP-2, that act with partners ZHP-3 and ZHP-4 to ensure the formation of a single crossover per chromosome, localize to short arms and are required for asymmetric SC disassembly [15] . In addition, phosphoregulation of the SC transverse and central elements, SYP-1 and SYP-2, is known to promote establishment of short and long arms [16,17] . MAP kinase-mediated phosphorylation of SYP-2 and subsequent inactivation of MAPK upon crossover designation triggers disassembly of SC central element proteins from the long arm [17] .…”

mentioning

confidence: 99%

“…Phosphorylation at the Polo Box Domain (PBD) binding motif of SYP-1 at Thr452 promotes the cascade of short and long arm establishment by recruiting PLK-2 to the SC. Phosphorylated SYP-1 and PLK-2 are mutually dependent for their colocalization on short arms upon crossover designation, and a non-phosphorylatable syp-1 mutation leads to loss of asymmetry and failure in meiosis I segregation [16] . Once short/long asymmetry is established, the chromosome passenger complex (CPC) containing INCENP ICP-1 and Aurora B AIR-2 is recruited to the short arm by Haspin kinase phosphorylation of histone H3Thr3 [16,[18][19][20] .…”

mentioning

confidence: 99%

“…Phosphorylated SYP-1 and PLK-2 are mutually dependent for their colocalization on short arms upon crossover designation, and a non-phosphorylatable syp-1 mutation leads to loss of asymmetry and failure in meiosis I segregation [16] . Once short/long asymmetry is established, the chromosome passenger complex (CPC) containing INCENP ICP-1 and Aurora B AIR-2 is recruited to the short arm by Haspin kinase phosphorylation of histone H3Thr3 [16,[18][19][20] . H3Thr3 in turn is dephosphorylated on the long arm by HTP-1/LAB-1-based recruitment of phosphatase PP1 [18,21] .…”

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confidence: 99%

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Phosphoregulation of HORMA domain protein HIM-3 promotes asymmetric synaptonemal complex disassembly in meiotic prophase inC. elegans

Sato-Carlton

Tabuchi

et al. 2020

Preprint

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AbstractIn the two cell divisions of meiosis, diploid genomes are reduced into complementary haploid sets through the discrete, two-step removal of chromosome cohesion, a task carried out in most eukaryotes by protecting cohesion at the centromere until the second division. In eukaryotes without defined centromeres, however, alternative strategies have been innovated. The best-understood of these is that used by the nematode Caenorhabditis elegans, where upon division of the chromosome into two segments or arms by the single off-center crossover, several chromosome-associated proteins or post-translational modifications become specifically partitioned to either the short or long arm, where they affect the timing of cohesion loss through as-yet unknown mechanisms. Here, we investigate the meiotic axis HORMA-domain protein HIM-3 and show that it becomes phosphorylated at its C-terminus, within the conserved “closure motif” region bound by the related HORMA-domain proteins HTP-1 and HTP-2. Binding of HTP-2 is abrogated by phosphorylation of the closure motif in in vitro assays, strongly suggesting that in vivo phosphorylation of HIM-3 likely modulates the hierarchical structure of the chromosome axis. Phosphorylation of HIM-3 only occurs on synapsed chromosomes, and similarly to previously-described phosphorylated proteins of the synaptonemal complex, becomes restricted to the short arm after designation of crossover recombination sites. Regulation of HIM-3 phosphorylation status is required for timely disassembly of synaptonemal complex central elements from the long arm, and is also required for proper timing of HTP-1 and HTP-2 dissociation from the short arm. Phosphorylation of HIM-3 thus plays a role in establishing the identity of short and long arms, thereby contributing to the robustness of the two-step chromosome segregation.

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Section: Him-3 Hormad1/2 Is Phosphorylated At the Conserved Closure Mmentioning

confidence: 99%

Section: Phosphorylated Him-3 Localizes To the Entire Length Of The Smentioning

confidence: 99%

mentioning

confidence: 99%

mentioning

confidence: 99%

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confidence: 99%

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Phosphoregulation of HORMA domain protein HIM-3 promotes asymmetric synaptonemal complex disassembly in meiotic prophase inC. elegans

Sato-Carlton

Tabuchi

et al. 2020

Preprint

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X chromosome and autosomal recombination are differentially sensitive to disruptions in SC maintenance

Billmyre

Cahoon

Heenan

et al. 2019

Proc. Natl. Acad. Sci. U.S.A.

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The synaptonemal complex (SC) is a conserved meiotic structure that regulates the repair of double-strand breaks (DSBs) into crossovers or gene conversions. The removal of any central-region SC component, such as the Drosophila melanogaster transverse filament protein C(3)G, causes a complete loss of SC structure and crossovers. To better understand the role of the SC in meiosis, we used CRISPR/Cas9 to construct 3 in-frame deletions within the predicted coiled-coil region of the C(3)G protein. Since these 3 deletion mutations disrupt SC maintenance at different times during pachytene and exhibit distinct defects in key meiotic processes, they allow us to define the stages of pachytene when the SC is necessary for homolog pairing and recombination during pachytene. Our studies demonstrate that the X chromosome and the autosomes display substantially different defects in pairing and recombination when SC structure is disrupted, suggesting that the X chromosome is potentially regulated differently from the autosomes.

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Targeting Polo-like kinase in space and time during C. elegans meiosis

Brandt

Kim

2021

Cell Cycle

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A central player in meiotic chromosome dynamics is the conserved Polo-like kinase (PLK) family. PLKs are dynamically localized to distinct structures during meiotic prophase and phosphorylate a diverse group of substrates to control homolog pairing, synapsis, and meiotic recombination. In a recent study, we uncovered the mechanisms that control the targeting of a meiosis-specific PLK-2 in C. elegans. In early meiotic prophase, PLK-2 localizes to special chromosome regions known as pairing centers and drives homolog pairing and synapsis. PLK-2 then relocates to the synaptonemal complex (SC) after crossover designation and mediates chromosome remodeling required for homolog separation. What controls this intricate targeting of PLK-2 in space and time? We discuss recent findings and remaining questions for the future.

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Phosphorylation of the synaptonemal complex protein SYP-1 promotes meiotic chromosome segregation

Cited by 12 publications

References 69 publications

Phosphoregulation of HORMA domain protein HIM-3 promotes asymmetric synaptonemal complex disassembly in meiotic prophase inC. elegans

Phosphoregulation of HORMA domain protein HIM-3 promotes asymmetric synaptonemal complex disassembly in meiotic prophase inC. elegans

X chromosome and autosomal recombination are differentially sensitive to disruptions in SC maintenance

Targeting Polo-like kinase in space and time during C. elegans meiosis

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