Your search keyword '"Jordana C. Bloom"' showing total 13 results

1. Imaging optically thick tissues simply and reproducibly: a practical guide to Lightsheet Macroscopy

Author

Rebecca M. Williams, Jordana C. Bloom, Cara Robertus, Andrew K. Recknagel, David Putnam, John C. Schimenti, and Warren R. Zipfel

Abstract

Lightsheet microscopy offers an ideal method for imaging of large (mm-cm scale) biological tissues rendered transparent via optical clearing protocols. However the diversity of clearing technologies and tissue types, and how these are adapted to the microscope can make tissue mounting glitchy and somewhat irreproducible. Tissue preparation for imaging can involve glues and or equilibration in a variety of expensive and/or proprietary formulations. Here we present practical advice for mounting and capping cleared tissues in optical cuvettes for macroscopic imaging, providing a standardized 3D cell that can be imaged routinely and relatively inexpensively. We show that acrylic cuvettes should be non-aberrating with objective numerical apertures less than 0.65, and present an inexpensive tool for alignment and calibration of standard lightsheet parameters. Mouse embryo, liver and heart imaging are demonstrated as examples with practical recommendations for acquisition and post-processing.

Published

2022

2. Oocyte Elimination Through DNA Damage Signaling from CHK1/CHK2 to p53 and p63

Author

John C. Schimenti, Jordana C. Bloom, and Vera D. Rinaldi

Subjects

Male, DNA damage, Cell Cycle Proteins, Investigations, Biology, medicine.disease_cause, Mice, 03 medical and health sciences, 0302 clinical medicine, Prophase, Meiosis, Genetics, Homologous chromosome, medicine, Animals, CHEK1, Checkpoint Kinase 2, 030304 developmental biology, Mice, Knockout, 0303 health sciences, Mutation, Endodeoxyribonucleases, fungi, Synapsis, Cell biology, Chromosome Pairing, enzymes and coenzymes (carbohydrates), 030220 oncology & carcinogenesis, Checkpoint Kinase 1, Oocytes, Trans-Activators, ATPases Associated with Diverse Cellular Activities, Female, Tumor Suppressor Protein p53, biological phenomena, cell phenomena, and immunity, DNA Damage, Signal Transduction

Abstract

Unrepaired DNA damage in mouse oocytes leads to apoptosis, in part via CHK2 signaling to TRP53 and TRP63. Here, Rinaldi, Bloom, and Schimenti provide evidence that CHK1 can also be involved, especially... Eukaryotic organisms have evolved mechanisms to prevent the accumulation of cells bearing genetic aberrations. This is especially crucial for the germline, because fecundity and fitness of progeny would be adversely affected by an excessively high mutational incidence. The process of meiosis poses unique problems for mutation avoidance because of the requirement for SPO11-induced programmed double-strand breaks (DSBs) in recombination-driven pairing and segregation of homologous chromosomes. Mouse meiocytes bearing unrepaired meiotic DSBs or unsynapsed chromosomes are eliminated before completing meiotic prophase I. In previous work, we showed that checkpoint kinase 2 (CHK2; CHEK2), a canonical DNA damage response protein, is crucial for eliminating not only oocytes defective in meiotic DSB repair (e.g., Trip13Gt mutants), but also Spo11−/− oocytes that are defective in homologous chromosome synapsis and accumulate a threshold level of spontaneous DSBs. However, rescue of such oocytes by Chk2 deficiency was incomplete, raising the possibility that a parallel checkpoint pathway(s) exists. Here, we show that mouse oocytes lacking both p53 (TRP53) and the oocyte-exclusive isoform of p63, TAp63, protects nearly all Spo11−/− and Trip13Gt/Gt oocytes from elimination. We present evidence that checkpoint kinase I (CHK1; CHEK1), which is known to signal to TRP53, also becomes activated by persistent DSBs in oocytes, and to an increased degree when CHK2 is absent. The combined data indicate that nearly all oocytes reaching a threshold level of unrepaired DSBs are eliminated by a semiredundant pathway of CHK1/CHK2 signaling to TRP53/TAp63.

Published

2020

3. Female-biased embryonic death from genomic instability-induced inflammation

Author

Marsha D. Wallace, Jordana C. Bloom, Chen-Hua Chuang, Adrian J. McNairn, and John C. Schimenti

Subjects

0301 basic medicine, Genome instability, Male, Placenta, Mutant, Ibuprofen, medicine.disease_cause, Mice, 0302 clinical medicine, Pregnancy, Receptors, Interleukin-10, Testosterone, FANCM, Mutation, 0303 health sciences, Sex Characteristics, Multidisciplinary, Minichromosome Maintenance Proteins, Anti-Inflammatory Agents, Non-Steroidal, Sex reversal, 3. Good health, Cell biology, 030220 oncology & carcinogenesis, Embryo Loss, Female, Senescence, DNA Replication, DNA damage, Embryonic Development, Biology, Genomic Instability, Article, 03 medical and health sciences, Minichromosome maintenance, parasitic diseases, medicine, Animals, Gene, 030304 developmental biology, Cell Proliferation, Inflammation, DNA replication, DNA Helicases, Embryonic stem cell, Minichromosome Maintenance Complex Component 4, 030104 developmental biology, Synthetic Lethal Mutations, 030217 neurology & neurosurgery, DNA Damage

Abstract

Genomic instability can trigger cellular responses that include checkpoint activation, senescence and inflammation1,2. Although genomic instability has been extensively studied in cell culture and cancer paradigms, little is known about its effect during embryonic development, a period of rapid cellular proliferation. Here we report that mutations in the heterohexameric minichromosome maintenance complex—the DNA replicative helicase comprising MCM2 to MCM73,4—that cause genomic instability render female mouse embryos markedly more susceptible than males to embryonic lethality. This bias was not attributable to X chromosome-inactivation defects, differential replication licensing or X versus Y chromosome size, but rather to ‘maleness’—XX embryos could be rescued by transgene-mediated sex reversal or testosterone administration. The ability of exogenous or endogenous testosterone to protect embryos was related to its anti-inflammatory properties5. Ibuprofen, a non-steroidal anti-inflammatory drug, rescued female embryos that contained mutations in not only the Mcm genes but also the Fancm gene; similar to MCM mutants, Fancm mutant embryos have increased levels of genomic instability (measured as the number of cells with micronuclei) from compromised replication fork repair6. In addition, deficiency in the anti-inflammatory IL10 receptor was synthetically lethal with the Mcm4Chaos3 helicase mutant. Our experiments indicate that, during development, DNA damage associated with DNA replication induces inflammation that is preferentially lethal to female embryos, because male embryos are protected by high levels of intrinsic testosterone. Genomic instability, caused by MCM mutations, results in embryonic lethality that disproportionally affects female mouse embryos and is rescued by testosterone or ibuprofen treatment, both of which ameliorate inflammatory effects.

Published

2019

4. Sexually dimorphic DNA damage responses and mutation avoidance in the mouse germline

Author

Jordana C. Bloom and John C. Schimenti

Subjects

Male, endocrine system, DNA damage, Somatic cell, Piwi-interacting RNA, Endogeny, Biology, Embryonic Germ Cells, medicine.disease_cause, Germline, 03 medical and health sciences, Mice, 0302 clinical medicine, Sex Factors, Pregnancy, Radiation, Ionizing, Genetics, medicine, Animals, RNA, Small Interfering, 030304 developmental biology, 0303 health sciences, Mutation, urogenital system, fungi, Cell Differentiation, Cell Cycle Checkpoints, DNA, Cell biology, Meiosis, medicine.anatomical_structure, Germ Cells, 030220 oncology & carcinogenesis, embryonic structures, DNA Transposable Elements, Oocytes, Exogenous DNA, Female, Germ cell, Developmental Biology, Research Paper, DNA Damage

Abstract

Germ cells specified during fetal development form the foundation of the mammalian germline. These primordial germ cells (PGCs) undergo rapid proliferation, yet the germline is highly refractory to mutation accumulation compared to somatic cells. Importantly, while the presence of endogenous or exogenous DNA damage has the potential to impact PGCs, there is little known about how these cells respond to stressors. To better understand the DNA damage response (DDR) in these cells, we exposed pregnant mice to ionizing radiation (IR) at specific gestational time points and assessed the DDR in PGCs. Our results show that PGCs prior to sex determination lack a G1 cell cycle checkpoint. Additionally, the response to IR-induced DNA damage differs between female and male PGCs post-sex determination. IR of female PGCs caused uncoupling of germ cell differentiation and meiotic initiation, while male PGCs exhibited repression of piRNA metabolism and transposon de-repression. We also used whole genome single-cell DNA sequencing to reveal that genetic rescue of DNA repair-deficient germ cells (Fancm-/-) leads to increased mutation incidence and biases. Importantly, our work uncovers novel insights into how PGCs exposed to DNA damage can become developmentally defective, leaving only those genetically fit cells to establish the adult germline.

Published

2020

5. Single Cell Analysis Reveals Multi-faceted miR-375 Regulation of the Intestinal Crypt

Author

Jordana C. Bloom, Matt Kanke, Nicolas Buchon, Michael J. Shanahan, Bailey C.E. Peck, Rebecca L. Cubitt, Lukas E. Dow, Breanna Sheahan, Shengli Ding, Wendy A. Pitman, Alessandro Bonfini, Praveen Sethupathy, Christopher M. Dekaney, Vera D. Rinaldi, Ennessa G. Curry, Elia D. Tait-Wojno, Ajeet Singh, Oyebola O. Oyesola, Adrian J. McNairn, Yu-Han Hung, Jonathan W. Villanueva, and John C. Schimenti

Subjects

YAP1, Single-cell analysis, Mir-375, Gene expression, Crypt, microRNA, Tuft cell, Stem cell, Biology, Cell biology

Abstract

SummaryThe role of individual miRNAs in small intestinal (SI) epithelial homeostasis is under-explored. In this study, we discovered that miR-375 is among the most enriched miRNAs in intestinal crypts and stem cells (ISCs), especially facultative ISCs. We then showed by multiple manipulations, including CRISPR/Cas9 editing, that miR-375 is strongly suppressed by Wnt-signaling. Single-cell RNA-seq analysis of SI crypt-enriched cells from miR-375 knockout (375-KO) mice revealed elevated numbers of tuft cells and increased expression of pro-proliferative genes in ISCs. Accordingly, the genetic loss of miR-375 promoted resistance to helminth infection and enhanced the regenerative response to irradiation. The conserved effects of miR-375 were confirmed by gain-of-function studies in Drosophila midgut stem cells in vivo. Moreover, functional experiments in enteroids uncovered a regulatory relationship between miR-375 and Yap1 that controls cell survival. Finally, analysis of mouse model and clinical data revealed an inverse association between miR-375 levels and intestinal tumor development.HighlightsmiR-375 is one of the most enriched miRNAs in ISCs, especially facultative ISCs.miR-375 modifies tuft cell abundance and pro-proliferative gene expression in ISCs.Loss of miR-375 in mice enhances the host response to helminth infection and crypt regeneration.Mouse and human intestinal cancer are associated with reduced miR-375 expression.eTOC BlurbSethupathy and colleagues show that miR-375 is a Wnt-responsive, ISC-enriched miRNA that serves as a break on intestinal crypt proliferation. They also show that miR-375 modulates tuft cell abundance and pro-proliferative gene expression in ISCs, that miR-375 loss enhances the host response to helminth infection as well as crypt regeneration post-irradiation, and its reduced expression is associated with intestinal cancer.

Published

2020

6. A reporter mouse for in vivo detection of<scp>DNA</scp>damage in embryonic germ cells

Author

John C. Schimenti and Jordana C. Bloom

Subjects

Male, Embryonic Germ Cells, DNA repair, DNA damage, Transgene, Endogeny, Biology, Article, Mice, 03 medical and health sciences, chemistry.chemical_compound, 0302 clinical medicine, Endocrinology, Genes, Reporter, Genetics, Animals, DNA Breaks, Double-Stranded, 030304 developmental biology, 0303 health sciences, Cell Biology, Chromatin, Cell biology, Mice, Inbred C57BL, Luminescent Proteins, chemistry, Female, Exogenous DNA, Genetic Engineering, Octamer Transcription Factor-3, 030217 neurology & neurosurgery, DNA, DNA Damage, Protein Binding

Abstract

Maintaining genome integrity in the germline is essential for survival and propagation of a species. In both mouse and human, germ cells originate during fetal development and are hypersensitive to both endogenous and exogenous DNA damaging agents. Currently, mechanistic understanding of how primordial germ cells respond to DNA damage is limited in part by the tools available to study these cells. We developed a mouse transgenic reporter strain expressing a 53BP1-mCherry fusion protein under the control of the Oct4ΔPE embryonic germ cell-specific promoter. This reporter binds sites of DNA double strand breaks (DSBs) on chromatin, forming foci. Using ionizing radiation as a DNA double strand break-inducing agent, we show that the transgenic reporter expresses specifically in the embryonic germ cells of both sexes and forms DNA damage induced foci in both a dose- and time-dependent manner. The dynamic time-sensitive and dose-sensitive DNA damage detection ability of this transgenic reporter, in combination with its specific expression in embryonic germ cells, makes it a versatile and valuable tool for increasing our understanding of DNA damage responses in these unique cells.

Published

2020

7. Mouse Genetics 2016: meeting report

Author

Jordana C. Bloom, Robert J. Yamulla, and Tina N. Tran

Subjects

0301 basic medicine, 03 medical and health sciences, 030104 developmental biology, Genetics, Computational biology, Biology, Human genetics

Published

2017

8. Signaling to TRP53 and TAp63 from CHK1/CHK2 is responsible for elimination of most oocytes defective for either chromosome synapsis or recombination

Author

John C. Schimenti, Jordana C. Bloom, and Vera D. Rinaldi

Subjects

0303 health sciences, Mutation, DNA damage, fungi, Synapsis, Biology, medicine.disease_cause, Cell biology, enzymes and coenzymes (carbohydrates), 03 medical and health sciences, 0302 clinical medicine, Prophase, Meiosis, Homologous chromosome, medicine, CHEK1, biological phenomena, cell phenomena, and immunity, Checkpoint Kinase 2, 030217 neurology & neurosurgery, 030304 developmental biology

Abstract

Eukaryotic organisms have evolved mechanisms to prevent the accumulation of cells bearing genetic aberrations. This is especially crucial for the germline, because fecundity, and fitness of progeny would be adversely affected by an excessively high mutational incidence. The process of meiosis poses unique problems for mutation avoidance, due to the requirement for SPO11-induced programmed double strand breaks (DSBs) in recombination-driven pairing and segregation of homologous chromosomes. Mouse meiocytes bearing unrepaired meiotic DSBs or unsynapsed chromosomes are eliminated before completing meiotic prophase I. In previous work, we showed that checkpoint kinase 2 (CHK2; CHEK2), a canonical DNA damage response protein, is crucial for eliminating not only oocytes defective in meiotic DSB repair (e.g.Trip13Gtmutants), but also asynapticSpo11−/−oocytes that accumulate a threshold level of spontaneous DSBs. However, rescue of such oocytes byChk2deficiency was incomplete, raising the possibility that a parallel checkpoint pathway(s) exists. Here, we show that mouse oocytes lacking both TAp63 and TRP53 protects nearly allSpo11−/−andTrip13Gt/Gtoocytes from elimination. We present evidence that checkpoint kinase I (CHK1; CHEK1), which is known to signal to TRP53, also becomes activated by persistent DSBs in oocytes, and to an increased degree when CHK2 is absent. The combined data indicate that nearly all oocytes reaching a threshold level of unrepaired DSBs are eliminated by a semi-redundant pathway of CHK1/CHK2 signaling to TRP53/TAp63.

Published

2019

9. Germline genome protection: implications for gamete quality and germ cell tumorigenesis

Author

Amanda R Loehr, Robert S. Weiss, Jordana C. Bloom, and John C. Schimenti

Subjects

endocrine system, DNA repair, Somatic cell, Urology, Endocrinology, Diabetes and Metabolism, Testicular Germ Cell Tumor, Embryonic Germ Cells, Biology, medicine.disease_cause, Article, Germline, 03 medical and health sciences, 0302 clinical medicine, Endocrinology, Testicular Neoplasms, medicine, Animals, Humans, Induced pluripotent stem cell, 030219 obstetrics & reproductive medicine, Neoplasms, Germ Cell and Embryonal, Cell cycle, medicine.anatomical_structure, Reproductive Medicine, Drug Resistance, Neoplasm, Cancer research, Carcinogenesis, Germ cell, DNA Damage

Abstract

BACKGROUND Germ cells have a unique and critical role as the conduit for hereditary information and therefore employ multiple strategies to protect genomic integrity and avoid mutations. Unlike somatic cells, which often respond to DNA damage by arresting the cell cycle and conducting DNA repair, germ cells as well as long-lived pluripotent stem cells typically avoid the use of error-prone repair mechanisms and favor apoptosis, reducing the risk of genetic alterations. Testicular germ cell tumors, the most common cancers of young men, arise from pre-natal germ cells. OBJECTIVES To summarize the current understanding of DNA damage response mechanisms in pre-meiotic germ cells and to discuss how they impact both the origins of testicular germ cell tumors and their remarkable responsiveness to genotoxic chemotherapy. MATERIALS AND METHODS We conducted a review of literature gathered from PubMed regarding the DNA damage response properties of testicular germ cell tumors and the germ cells from which they arise, as well as the influence of these mechanisms on therapeutic responses by testicular germ cell tumors. RESULTS AND DISCUSSION This review provides a comprehensive evaluation of how the developmental origins of male germ cells and their inherent germ cell-like DNA damage response directly impact the development and therapeutic sensitivity of testicular germ cell tumors. CONCLUSIONS The DNA damage response of germ cells directly impacts the development and therapeutic sensitivity of testicular germ cell tumors. Recent advances in the study of primordial germ cells, post-natal mitotically dividing germ cells, and pluripotent stem cells will allow for new investigations into the initiation, progression, and treatment of testicular germ cell tumors.

Published

2019

10. Nuclear RNR-α Antagonizes Cell Proliferation by Directly Inhibiting ZRANB3

Author

Yuan Fu, Marcus J. C. Long, Jordana C. Bloom, Somsinee Wisitpitthaya, Islam M. Elsaid, Robert S. Weiss, Huma Inayat, Yimon Aye, Timothy M. Pierpont, and Joaquin Ortega

Subjects

0301 basic medicine, DNA Replication, DNA damage, Active Transport, Cell Nucleus, Article, 03 medical and health sciences, Mice, 0302 clinical medicine, Cytosol, Chlorocebus aethiops, Ribonucleotide Reductases, Animals, Humans, RNA, Small Interfering, Molecular Biology, Cell Proliferation, Cell Nucleus, DNA synthesis, Cell growth, Chemistry, Cell Cycle, DNA replication, DNA Helicases, Cell Biology, DNA, Cell cycle, Fibroblasts, Cell biology, 030104 developmental biology, Ribonucleotide reductase, HEK293 Cells, Mutagenesis, 030220 oncology & carcinogenesis, COS Cells, Mutation, NIH 3T3 Cells, Signal transduction, Nuclear transport, K562 Cells, DNA Damage, HeLa Cells, Protein Binding, Signal Transduction

Abstract

Since the origins of DNA-based life, the enzyme ribonucleotide reductase (RNR) has spurred proliferation because of its rate-limiting role in de novo deoxynucleoside-triphosphate (dNTP) biosynthesis. Paradoxically, the large subunit, RNR-α, of this obligatory two-component complex in mammals plays a context-specific anti-proliferative role. There is little explanation for this dichotomy. Here, we show that RNR-αhas a previously-unrecognized DNA-replication-inhibition function, leading to growth retardation. This underappreciated biological activity functions in the nucleus where RNR-α interacts with ZRANB3. This process suppresses ZRANB3’s function in unstressed cells that we show to be promotion of DNA-synthesis. This non-reductase-function of RNR-α is promoted by RNR-α-hexamerization—induced by natural- and synthetic-nucleotide of dA/ClF/CLA/FLU—which elicits rapid RNR-α nuclear import. The newly-discovered nuclear signaling axis is a primary defense against elevated/imbalanced dNTP-pools that can exert mutagenic effects irrespective of the cell cycle.

Published

2018

11. Whole Mount Immunofluorescence and Follicle Quantification of Cultured Mouse Ovaries

Author

Jordana C. Bloom, John C. Schimenti, and Vera D. Rinaldi

Subjects

0301 basic medicine, General Chemical Engineering, Cell Culture Techniques, Fluorescent Antibody Technique, Ovary, Biology, Immunofluorescence, General Biochemistry, Genetics and Molecular Biology, 03 medical and health sciences, Follicle, Mice, Ovarian Follicle, Reproductive biology, medicine, Animals, Ovarian follicle, Tissue clearing, medicine.diagnostic_test, General Immunology and Microbiology, General Neuroscience, Oocyte, Cell biology, 030104 developmental biology, medicine.anatomical_structure, Cell culture, Female, Developmental Biology

Abstract

Research in the field of mammalian reproductive biology often involves evaluating the overall health of ovaries and testes. Specifically, in females, ovarian fitness is often assessed by visualizing and quantifying follicles and oocytes. Because the ovary is an opaque three-dimensional tissue, traditional approaches require laboriously slicing the tissue into numerous serial sections in order to visualize cells throughout the entire organ. Furthermore, because quantification by this method typically entails scoring only a subset of the sections separated by the approximate diameter of an oocyte, it is prone to inaccuracy. Here, a protocol is described that instead utilizes whole organ tissue clearing and immunofluorescence staining of mouse ovaries to visualize follicles and oocytes. Compared to more traditional approaches, this protocol is advantageous for visualizing cells within the ovary for numerous reasons: 1) the ovary remains intact throughout sample preparation and processing; 2) small ovaries, which are difficult to section, can be examined with ease; 3) cellular quantification is more readily and accurately achieved; and 4) the whole organ imaged.

Published

2018

12. SMG-ly knocking out gene expression in specific cells: an educational primer for use with 'a novel strategy for cell-autonomous gene knockdown in caenorhabditis elegans defines a cell-specific function for the G-protein subunit GOA-1'

Author

Jordana C. Bloom and Philip M. Meneely

Subjects

Genetics, Gene knockdown, education, biology, cell-specific gene expression, Protein subunit, Nonsense-mediated decay, GTP-Binding Protein alpha Subunits, Gi-Go, nonsense-mediated decay (NMD), biology.organism_classification, Primer, Nonsense Mediated mRNA Decay, Gene Knockdown Techniques, Gene expression, Animals, Primer (molecular biology), Caenorhabditis elegans, Caenorhabditis elegans Proteins, Function (biology)

Abstract

SUMMARY A recent article by Maher et al. in GENETICS introduces an alternative approach to cell-type-specific gene knockdown in Caenorhabditis elegans, using nonsense-mediated decay. This strategy has the potential to be applicable to other organisms (this strategy requires that animals can survive without nonsense-mediated decay—not all can). This Primer article provides a guide and resource for educators and students by describing different gene knockdown methodologies, by assisting with the technically difficult portions of the Maher et al. article, and by providing conceptual questions relating to the article. Related article in GENETICS: Maher, K. N., A. Swaminathan, P. Patel, and D. L. Chase, 2013 A novel strategy for cell-autonomous gene knockdown in Caenorhabditis elegans defines a cell-specific function for the G-protein subunit GOA-1. Genetics 194: 363–373.

Published

2013

13. SKP1 drives the prophase I to metaphase I transition during male meiosis

Author

Michael A. Lampson, Lukáš Chmátal, Jordana C. Bloom, Mengcheng Luo, P. Jeremy Wang, N. Adrian Leu, Gordon Ruthel, Yongjuan Guan, John C. Schimenti, and Jun Ma

Subjects

Male, BUB1, Mice, Transgenic, Biology, PLK1, 03 medical and health sciences, Meiotic Prophase I, Mice, 0302 clinical medicine, Sex Factors, Meiosis, Centromere, Animals, Metaphase, S-Phase Kinase-Associated Proteins, Research Articles, Alleles, 030304 developmental biology, 0303 health sciences, Multidisciplinary, urogenital system, fungi, Synapsis, SciAdv r-articles, Cell Biology, Ubiquitin ligase, Cell biology, Gene Expression Regulation, 030220 oncology & carcinogenesis, Mesothelin, biology.protein, Oocytes, Research Article, Developmental Biology

Abstract

SKP1 coordinates chromosome synapsis and meiotic recombination with progression through the first meiotic cell division in mouse., The meiotic prophase I to metaphase I (PI/MI) transition requires chromosome desynapsis and metaphase competence acquisition. However, control of these major meiotic events is poorly understood. Here, we identify an essential role for SKP1, a core subunit of the SKP1–Cullin–F-box (SCF) ubiquitin E3 ligase, in the PI/MI transition. SKP1 localizes to synapsed chromosome axes and evicts HORMAD proteins from these regions in meiotic spermatocytes. SKP1-deficient spermatocytes display premature desynapsis, precocious pachytene exit, loss of PLK1 and BUB1 at centromeres, but persistence of HORMAD, γH2AX, RPA2, and MLH1 in diplonema. Strikingly, SKP1-deficient spermatocytes show sharply reduced MPF activity and fail to enter MI despite treatment with okadaic acid. SKP1-deficient oocytes exhibit desynapsis, chromosome misalignment, and progressive postnatal loss. Therefore, SKP1 maintains synapsis in meiosis of both sexes. Furthermore, our results support a model where SKP1 functions as the long-sought intrinsic metaphase competence factor to orchestrate MI entry during male meiosis.