Sister chromatid cohesion, mediated by a complex called cohesin, is crucial--particularly at centromeres--for proper chromosome segregation in mitosis and meiosis. In animal mitotic cells, phosphorylation of cohesin promotes its dissociation from chromosomes, but centromeric cohesin is protected by shugoshin until kinetochores are properly captured by the spindle microtubules. However, the mechanism of shugoshin-dependent protection of cohesin is unknown. Here we find a specific subtype of serine/threonine protein phosphatase 2A (PP2A) associating with human shugoshin. PP2A colocalizes with shugoshin at centromeres and is required for centromeric protection. Purified shugoshin complex has an ability to reverse the phosphorylation of cohesin in vitro, suggesting that dephosphorylation of cohesin is the mechanism of protection at centromeres. Meiotic shugoshin of fission yeast also associates with PP2A, with both proteins collaboratively protecting Rec8-containing cohesin at centromeres. Thus, we have revealed a conserved mechanism of centromeric protection of eukaryotic chromosomes in mitosis and meiosis.
Chromosome structure is dynamically regulated during cell division, and this regulation is dependent, in part, on condensin. The localization of condensin at chromosome arms is crucial for chromosome partitioning during anaphase. Condensin is also enriched at kinetochores but its precise role and loading machinery remain unclear. Here we show that fission yeast (Schizosaccharomyces pombe) kinetochore proteins Pcs1 and Mde4--homologues of budding yeast (Saccharomyces cerevisiae) monopolin subunits and known to prevent merotelic kinetochore orientation--act as a condensin 'recruiter' at kinetochores, and that condensin itself may act to clamp microtubule binding sites during metaphase. In addition to the regional recruitment factors, overall condensin association with chromatin is governed by the chromosomal passenger kinase Aurora B. Aurora-B-dependent phosphorylation of condensin promotes its association with histone H2A and H2A.Z, which we identify as conserved chromatin 'receptors' of condensin. Condensin phosphorylation and its deposition onto chromosome arms reach a peak during anaphase, when Aurora B kinase relocates from centromeres to the spindle midzone, where the separating chromosome arms are positioned. Our results elucidate the molecular basis for the spatiotemporal regulation of mitotic chromosome architecture, which is crucial for chromosome partitioning.
The centromere of a chromosome is composed mainly of two domains, a kinetochore assembling core centromere and peri-centromeric heterochromatin regions. The crucial role of centromeric heterochromatin is still unknown, because even in simpler unicellular organisms such as the fission yeast Schizosaccharomyces pombe, the heterochromatin protein Swi6 (HP1 homologue) has several functions at centromeres, including silencing gene expression and recombination, enriching cohesin, promoting kinetochore assembly, and, ultimately, preventing erroneous microtubule attachment to the kinetochores. Here we show that the requirement of heterochromatin for mitotic chromosome segregation is largely replaced by forcibly enriching cohesin at centromeres in fission yeast. However, this enrichment of cohesin is not sufficient to replace the meiotic requirement for heterochromatin. We find that the heterochromatin protein Swi6 associates directly with meiosis-specific shugoshin Sgo1, a protector of cohesin at centromeres. A point mutation of Sgo1 (V242E), which abolishes the interaction with Swi6, impairs the centromeric localization and function of Sgo1. The forced centromeric localization of Sgo1 restores proper meiotic chromosome segregation in swi6 cells. We also show that the direct link between HP1 and shugoshin is conserved in human cells. Taken together, our findings suggest that the recruitment of shugoshin is the important primary role for centromeric heterochromatin in ensuring eukaryotic chromosome segregation.
During cell division microtubules capture chromosomes by binding to the kinetochore assembled in the centromeric region of chromosomes. In mitosis sister chromatids are captured by microtubules emanating from both spindle poles, a process called bipolar attachment, whereas in meiosis I sisters are attached to microtubules originating from one spindle pole, called monopolar attachment. For determining chromosome orientation, kinetochore geometry or structure might be an important target of regulation. However, the molecular basis of this regulation has remained elusive. Here we show the link between kinetochore orientation and cohesion within the centromere in fission yeast Schizosaccharomyces pombe by strategies developed to visualize the concealed cohesion within the centromere, and to introduce artificial tethers that can influence kinetochore geometry. Our data imply that cohesion at the core centromere induces the mono-orientation of kinetochores whereas cohesion at the peri-centromeric region promotes bi-orientation. Our study may reveal a general mechanism for the geometric regulation of kinetochores, which collaborates with previously defined tension-dependent reorientation machinery.
Therefore, a conserved mechanism for meiotic kinetochore regulation remains elusive.Here we have identified meiosis-specific kinetochore factor MEIKIN in mouse, which functions in meiosis I but neither in meiosis II nor in mitosis. MEIKIN plays a crucial role in both mono-orientation and centromeric cohesion protection, partly by stabilizing the localization of the cohesin protector shugoshin. These functions are mediated largely by the activity of Polo-like kinase PLK1, which is enriched to kinetochores depending on MEIKIN. Our integrative analysis indicates that MEIKIN is the long awaited key regulator of meiotic kinetochore function, which is conserved from yeasts to humans. 2In mitosis, sister chromatid cohesion is established depending on cohesin in S phase and maintained until metaphase when the sister chromatids are captured by spindle microtubules from opposite poles and aligned on the spindle equator. For the onset of anaphase, the anaphase-promoting complex (APC) triggers the degradation of securin, an inhibitory chaperone for separase that cleaves cohesin RAD21 and removes cohesin along the entire chromosome. This removal of cohesin triggers the separation of sister chromatids and their movement to opposite poles, a process called equational division [1][2][3] . During meiosis, however, meiotic cohesin REC8 largely replaces RAD21 along the entire chromosomes; one round of DNA replication is followed by two rounds of nuclear division, which results in four haploid nuclei or gametes (Fig. 1a).In the first division of meiosis (meiosis I), homologous chromosomes connected by chiasmata are captured from the opposite poles, while sisters are captured from the same pole (mono-orientation). At the onset of anaphase I, REC8 cohesin is cleaved by separase along the arm regions, but protected at centromeres until metaphase II 4-6 . Thus, mono-orientation and centromeric cohesion protection are two hallmarks of meiotic kinetochore function, which are widely conserved among eukaryotic organisms 7-9 (Fig. 1a). There is accumulating evidence that cohesion protection is mediated by the centromeric protein shugoshin (SGO) and its partner protein phosphatase 2A (PP2A) [10][11][12][13][14][15] , which antagonizes REC8 phosphorylation, a prerequisite of cleavage 16, 17 . So far, meiosis-specific kinetochore proteins have been identified only in two yeasts (S. cerevisiae Spo13 and Mam1 (monopolin subunit), and S. pombe Moa1) [18][19][20][21][22][23] . Puzzlingly, however, because their structural and functional similarities remain to be identified, conservation of meiotic kinetochore regulation is questionable even between yeasts 8, 9 . Therefore, in this study, we address the long-standing question of whether meiotic kinetochore regulation is conserved from yeasts to mammals, and, if so, how. Mammalian meiotic kinetochore protein MEIKINFission yeast Moa1 interacts directly with the conserved kinetochore protein Cnp3 (CENP-C homolog), and localizes to the kinetochore in meiosis I 24 . To identify an equivalent meiosis...
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