Meiosis-specific functions of kinetochore protein SPC105R required for chromosome segregation in Drosophila oocytes

Author:

Joshi Jay N.1,Changela Neha1,Mahal Lia1,Jang Janet1,Defosse Tyler1,Wang Lin-Ing1,Das Arunika1,Shapiro Joanatta G.1,McKim Kim1

Affiliation:

1. Waksman Institute and Department of Genetics, Rutgers, the State University of New Jersey, Piscataway, NJ 08854

Abstract

The reductional division of meiosis I requires the separation of chromosome pairs towards opposite poles. We have previously implicated the outer kinetochore protein SPC105R/KNL1 in driving meiosis I chromosome segregation through lateral attachments to microtubules and coorientation of sister centromeres. To identify the domains of SPC105R that are critical for meiotic chromosome segregation, an RNAi-resistant gene expression system was developed. We found that the SPC105R C-terminal domain (aa 1284-1960) is necessary and sufficient for recruiting NDC80 to the kinetochore and building the outer kinetochore. Furthermore, the C-terminal domain recruits BUBR1, which in turn recruits the cohesion protection proteins MEI-S332 and PP2A. Of the remaining 1283 amino acids, we found the first 473 are most important for meiosis. The first 123 amino acids of the N-terminal half of SPC105R contain the conserved SLRK and RISF motifs that are targets of PP1 and Aurora B kinase and are most important for regulating the stability of microtubule attachments and maintaining metaphase I arrest. The region between amino acids 124 and 473 are required for lateral microtubule attachments and biorientation of homologues, which are critical for accurate chromosome segregation in meiosis I.

Publisher

American Society for Cell Biology (ASCB)

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