Application of morphometric techniques to postnatal rat testes in organ culture: insights into testis growth

Schlatt, Stefan; Yang, Zhengwei; Meehan, Terri Ann; Kretser, D. M. De; Loveland, Kate L

doi:10.1007/s004419900084

Cited by 36 publications

(26 citation statements)

References 29 publications

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“…The steady increase in cyst diameter during the spermatogonial stages is solely due to the proliferation of spermatogonia and Sertoli cells, at least for the first nine divisions. Careful analysis of DNA synthesis data in organ-culture experiments of immature rat testes similarly reveal an inverse relationship between germ-cell and Sertoli-cell proliferation, such that germ-cell DNA synthesis is low when Sertoli-cell DNA synthesis is elevated and vice versa (Schlatt et al 1999). Furthermore, FSH regulates both Sertoli-cell and differentiating spermatogonial DNA synthesis (Boitani et al 1995, Schlatt et al 1999.…”

Section: Discussionmentioning

confidence: 99%

“…Careful analysis of DNA synthesis data in organ-culture experiments of immature rat testes similarly reveal an inverse relationship between germ-cell and Sertoli-cell proliferation, such that germ-cell DNA synthesis is low when Sertoli-cell DNA synthesis is elevated and vice versa (Schlatt et al 1999). Furthermore, FSH regulates both Sertoli-cell and differentiating spermatogonial DNA synthesis (Boitani et al 1995, Schlatt et al 1999. By extension then, one explanation could be that seasonal alternating patterns in PCNA immunoreactivity in Sertoli and germ cells in sharks reflect variations in gonadotrophin secretion and/or changes in cell-type-specific responses to gonadotrophin secretion in these immature cysts.…”

Section: Discussionmentioning

confidence: 99%

“…Studies primarily in adult rodents indicate that, of the numerous regulatory mechanisms present within the testis, density-dependent (De Rooij 2001, Tadokoro et al 2002 and hormone-controlled (Meachem et al 1999, Allan et al 2004) mechanisms are two of the major physiological regulators that control these processes in an age-dependent and spermatogonial-stage-dependent manner. In addition, data obtained from organ cultures of immature rodent testes indicate that developing Sertoli cells influence the cellpopulation dynamics of gonocytes, and undifferentiated and differentiated spermatogonia, and their further maturation, depending on the age of the Sertoli cell (Boitani et al 1993, 1995, Zhou et al 1993, De Rooij & Van Dissel-Emiliani 1997, Schlatt et al 1999. Our knowledge of the inter-relationships between the different stages of spermatogonia and the various stages of Sertoli cell development in vivo is incomplete.…”

Section: Introductionmentioning

confidence: 99%

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Stage and season effects on cell cycle and apoptotic activities of germ cells and Sertoli cells during spermatogenesis in the spiny dogfish (Squalus acanthias)

McClusky¹

2005

Reproduction

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To understand the processes involved in the spatial and temporal maturation of testicular cells in Squalus acanthias, we used standard morphometry, proliferating-cell nuclear antigen (PCNA) and terminal deoxynucleotidyl transferase-mediated dUTP nick end-labelling (TUNEL) immunohistochemistry. Except for immature spermatocysts (germinal zone, GZ; early-stage premeiotic, E-PrM), the number of cysts in all subsequent stages and the total number of cysts in the spermatogenic progression varied seasonally. The spermatogenic cycle spans about 2 years and is interrupted by germcell clone deletion via apoptosis at the mitosis-meiosis transition in April/May, manifesting as a zone of degeneration (ZD). Rate of displacement of the ZD across the testis diameter indicates that late-stage premeiotic (L-PrM) generations 12-13 require 9 -10 months to reach the mature-spermatid stage. Also, the number of cysts completing spermatogenesis is approximately 4-5-fold less than the number that entered spermatogenesis proper 2 years earlier. Pronounced gonocytogenesis in the germinal ridge was coincident with ZD formation in April/May, but it was absent in the fall when mature spermatogonial and meiotic activities had resumed. Whereas strong Sertoli cell PCNA immunoreactivity dominated the GZ cyst cell-cycle activities throughout the year, except during the spring/summer months, the spermatogonial-and Sertoli-cell PCNA indices in E-PrM cysts were inversely related. PCNA immunoreactivity in spermatocytes was seasonal and dependent on the stage of meiosis. TUNEL labelling was limited to spermatogonia and increased stage-dependently in the PrM region (L-PrM 5 mid-stage PrM @ E-PrM @ GZ), correlating with ZD formation, in a season-dependent manner. Results imply that effects of normal regulatory factors in Squalus are stage-and process-specific.

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Section: Discussionmentioning

confidence: 99%

Section: Discussionmentioning

confidence: 99%

Section: Introductionmentioning

confidence: 99%

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Stage and season effects on cell cycle and apoptotic activities of germ cells and Sertoli cells during spermatogenesis in the spiny dogfish (Squalus acanthias)

McClusky¹

2005

Reproduction

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“…BrdU incorporation into testicular cells at 3, 9 and 18 dpp was detected by immunohistochemistry as previously described (Schlatt et al 1999), with minor modifications as described below (see Fig 1A). In brief, slides bearing paraffin-embedded tissue sections were deparaffinized, rehydrated, and subjected to antigen retrieval in citrate buffer (0·1 M, pH 6; 90-95 C for 10 min then room temperature for 20 min).…”

Section: Proliferation Analysismentioning

confidence: 99%

Developmentally distinct in vivo effects of FSH on proliferation and apoptosis during testis maturation

Meachem¹,

Ruwanpura²,

Ziolkowski³

et al. 2005

Journal of Endocrinology

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The critical influence of follicle stimulating hormone (FSH) on male fertility relates both to its impact on Sertoli cell proliferation in perinatal life and to its influence on the synthesis of Sertoli cell-derived products essential for germ cell survival and function in the developing adult testis. The nature and timing of this shift of germ cells to their reliance on specific Sertoli cell-derived products are not defined. Based on existing data, it is apparent that the dominant function of FSH shifts between 9 and 18 day postpartum (dpp) during the first wave of spermatogenesis from driving Sertoli cell proliferation to support germ cells. To enable comprehensive analysis of the impact of acute in vivo FSH suppression on Sertoli and germ cell development, FSH was selectively suppressed in Sprague-Dawley rats by passive immunisation for 2 days and/or 4 days prior to testis collection at 3, 9 and 18 dpp. The 3 dpp samples displayed no measurable changes, while 4 days of FSH suppression decreased Sertoli cell proliferation and numbers in 9 dpp, but not 18 dpp, animals. In contrast, germ cell numbers were unaffected at 9 dpp but decreased at 18 dpp following FSH suppression, with a corresponding increase in germ cell apoptosis measured at 18 dpp. Sixty transcripts were measured as changed at 18 dpp in response to 4 days of FSH suppression, as assessed using Affymetrix microarrays. Some of these are known as Sertoli cell-derived FSH-responsive genes (e.g. StAR, cathepsin L, insulin-like growth factor binding protein-3), while others encode proteins involved in cell cycle and survival regulation (e.g. cyclin D1, scavenger receptor class B 1). These data demonstrate that FSH differentially affects Sertoli and germ cells in an age-dependent manner in vivo, promoting Sertoli cell mitosis at day 9, and supporting germ cell viability at day 18. This model has enabled identification of candidate genes that contribute to the FSH-mediated pathway by which Sertoli cells support germ cells.

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“…Suitable methods to quantify cell proliferation are available (e.g. Thoolen 1990;Schlatt et al . 1999;Sakai 2002), and the biological effect of this synthetic estrogen addresses an interesting biological and environmental problem.…”

Section: Introductionmentioning

confidence: 99%

Effect of 17‐α‐ethynylestradiol on germ cell proliferation in organ and primary culture of medaka (Oryzias latipes) testis

Song

Gutzeit

2003

Dev Growth Differ

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Organ cultures and primary cell cultures of medaka ( Oryzias latipes ) testis were compared with respect to cell viability and cell proliferation. The analysis by fluorescence microscopy and flow cytometry showed that in both cultures the cells remained viable for at least 1 day and cell proliferation could be analyzed reliably by BrdU incorporation. The proliferating cells were mostly spermatogonia located at the periphery of the testis in tissue sections. Both culture systems were used to study the effect of 17-␣ -ethynylestradiol on cell proliferation. The results obtained with organ and primary cultures were consistent: low concentrations (0.01 and 1 n M ) of synthetic estrogen stimulated cell proliferation slightly, while a higher concentration (100 n M ) had an inhibitory effect. Both culture methods are suitable for the analysis of substances that might interfere with germ cell proliferation or other functions in spermatogenesis.

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Application of morphometric techniques to postnatal rat testes in organ culture: insights into testis growth

Cited by 36 publications

References 29 publications

Stage and season effects on cell cycle and apoptotic activities of germ cells and Sertoli cells during spermatogenesis in the spiny dogfish (Squalus acanthias)

Stage and season effects on cell cycle and apoptotic activities of germ cells and Sertoli cells during spermatogenesis in the spiny dogfish (Squalus acanthias)

Developmentally distinct in vivo effects of FSH on proliferation and apoptosis during testis maturation

Effect of 17‐α‐ethynylestradiol on germ cell proliferation in organ and primary culture of medaka (Oryzias latipes) testis

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