The Whole Meiotic Process Can Occur in Vitro in Untransformed Rat Spermatogenic Cells

Staub, Christophe; Hue, Dominique; Nicolle, J.C.; Perrard-Sapori, Marie-Hélène; Segretain, Dominique; Durand, Philippe

doi:10.1006/excr.2000.4998

Cited by 86 publications

(92 citation statements)

References 26 publications

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“…However, the ratio provides evidence that the proportion of Sertolian tissue in testis samples may vary greatly according to the different experimental/pathological conditions, even when the number of Sertoli cells remains unchanged. Similar variations were observed whether clusterin mRNA level was measured by Northern blot analysis or by competitive RT-PCR with RNA competitors; the latter method is much more sensitive than the former, enabling analysis from small amounts of tissue such as from clinical biopsies or Sertoli/germ cell co-cultures (Weiss et al 1997, Staub et al 2000. The use of clusterin mRNA as a marker of the amount of RNA of Sertoli cell origin is, however, limited to rats of 20 days old or more, since immature Sertoli cells do not express clusterin mRNA levels as high as those of mature Sertoli cells.…”

Section: Discussionmentioning

confidence: 62%

“…In order to measure SCF and clusterin mRNA from small amounts of tissue, such as can be obtained from co-cultures of Sertoli and germ cells (Weiss et al 1997), seminiferous tubule cultures (Staub et al 2000) or testicular biopsies, we developed a competitive RT-PCR procedure that monitored both the reverse transcription and the PCR steps.…”

Section: Measurements Of Scf and Clusterin Mrna Levels By Competitivementioning

confidence: 99%

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Quantification of stem cell factor mRNA levels in the rat testis: usefulness of clusterin mRNA as a marker of the amount of mRNA of sertoli cell origin in post pubertal rats

Plotton¹,

Sanchez²,

Perrard³

et al. 2005

Journal of Endocrinology

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Spermatogenesis is a complex cellular process regulated by gonadotrophins and local cell-cell interactions. Stem cell factor (SCF) is one of the paracrine factors, produced by the Sertoli cells, involved in the local regulation of spermatogenesis. Measurement of its testicular level is important for addressing its role in testis physiopathology. However, the relative cell composition of experimental and pathological testis samples may lead to misinterpretation in relating SCF mRNA levels to the amount of RNA extracted from the whole tissue sample. Taking into account the relative RNA content of Sertoli cell origin should provide more significant data. In the present study, three sets of experiments were intended for modifying the proportion of RNA of Sertoli cell origin in RNA extracted from whole testis tissue samples: during postnatal development; following methoxy-acetic acid (MAA) administration; and after injecting a long-acting gonadotrophin-releasing hormone agonist (GnRHa). In a first step, we demonstrated clusterin mRNA level stability in purified Sertoli cell preparations between 20 days and adulthood, and following MAA or GnRHa treatment. In a second step, we used a competitive RT-PCR assay to measure SCF and clusterin mRNA levels and expressed the amount of SCF mRNA relative to the amount of clusterin mRNA under the above experimental conditions. The SCF/clusterin mRNA level ratio was found to remain roughly stable from 20 days post-partum to adulthood; i.e. during the development of spermatogenesis. MAA administration led to an overall increase in the SCF/clusterin mRNA level ratio between 7 and 14 days after administration, consistent with the replenishment of the testis with pachytene spermatocytes and round spermatids. Conversely, after long-acting GnRHa injection, the SCF/clusterin mRNA level ratio decreased only slightly from day 21 onward. Hence, the present studies indicate that, under physiopathological conditions, the amount of clusterin mRNA is a good marker of the amount of RNA of Sertoli cell origin in testis samples at day 20 or later; different experimental alterations of spermatogenesis are associated with different patterns of SCF mRNA levels; the relationship between FSH and SCF in vivo is not as simple as that described in vitro.

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Section: Discussionmentioning

confidence: 62%

Section: Measurements Of Scf and Clusterin Mrna Levels By Competitivementioning

confidence: 99%

Quantification of stem cell factor mRNA levels in the rat testis: usefulness of clusterin mRNA as a marker of the amount of mRNA of sertoli cell origin in post pubertal rats

Plotton¹,

Sanchez²,

Perrard³

et al. 2005

Journal of Endocrinology

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“…Seminiferous tubules were prepared as described previously (Guibert et al 2013) and seeded in static 24-well cell culture polyethylene terephthalate inserts (pore 0.4 µm, WWR, Fontenay sous Bois, France) as described previously (Djakiew & Dym 1988, Staub et al 2000, Legendre et al 2010. This was carried out in order to preserve germ cells on polarised Sertoli cells in a dynamic culture using the Quasi-Vivo system (Kirkstall Ltd, Rotherham, UK).…”

Section: Culture Of Chicken Seminiferous Tubulesmentioning

confidence: 99%

The insulin sensitiser metformin regulates chicken Sertoli and germ cell populations

Faure¹,

Guibert²,

Alves³

et al. 2016

Reproduction

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Metformin, an insulin sensitiser from the biguanide family of molecules, is used for the treatment of insulin resistance in type 2 diabetes individuals. It increases peripheral glucose uptake and may reduce food intake. Based on the tight link between metabolism and fertility, we investigated the role of metformin on testicular function using in vitro culture of Sertoli cells and seminiferous tubules, complemented by in vivo data obtained following metformin administration to prepubertal chickens. In vitro, metformin treatment reduced Sertoli cell proliferation without inducing apoptosis and morphological changes. The metabolism of Sertoli cells was affected because lactate secretion by Sertoli cells increased approximately twofold and intracellular free ATP was negatively impacted. Two important pathways regulating proliferation and metabolism in Sertoli cells were assayed. Metformin exposure was not associated with an increased phosphorylation of AKT or ERK. There was a 90% reduction in the proportion of proliferating germ cells after a 96-h exposure of seminiferous tubule cultures to metformin. In vivo, 6-week-old chickens treated with metformin for 3 weeks exhibited reduced testicular weight and a 50% decrease in testosterone levels. The expression of a marker of undifferentiated germ cells was unchanged in contrast to the decrease in expression of 'protamine', a marker of differentiated germ cells. In conclusion, these results suggest that metformin affects the testicular energy content and the proliferative ability of Sertoli and germ cells.

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“…To elucidate the mechanism of spermatogenesis and the conditions required for this process, researchers have long attempted to recapitulate the process in vitro [2,3]. Several reports have claimed to have achieved the completion of meiosis leading to the production of spermatids in vitro [4,5]. Those studies, however, have used the testicular cells of immature animals as experimental material, which include not only spermatogonial stem cells but also spermatocytes from the meiotic stage.…”

Section: Introductionmentioning

confidence: 99%

Ectopic porcine spermatogenesis in murine subcutis: tissue grafting versus cell-injection methods

Watanabe¹,

Hayashi²,

Kita³

et al. 2009

Asian J Androl

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Fragments of testis tissue from immature animals grow and develop spermatogenesis when grafted onto subcutaneous areas of immunodeficient mice. The same results are obtained when dissociated cells from immature testes of rodents are injected into the subcutis of nude mice. Those cells reconstitute seminiferous tubules and facilitate spermatogenesis. We compared these two methods, tissue grafting and cell-injection methods, in terms of the efficiency of spermatogenesis in the backs of three strains of immunodeficient mice, using neonatal porcine testicular tissues and cells as donor material. Nude, severe combined immunodeficient (SCID) and NOD/Shi-SCID, IL-2Rγ c null (NOG) mice were used as recipients. At 10 months after surgery, the transplants were examined histologically. Both grafting and cell-injection methods resulted in porcine spermatogenesis on the backs of recipient mice; the percentage of spermatids present in the transplants was 67% and 22%, respectively. Using the grafting method, all three strains of mice supported the same extent of spermatogenesis. As for the cellinjection method, although SCID mice were the best host for supporting reconstitution and spermatogenesis, any difference from the other strains was not significant. As NOG mice did not show any better results, the severity of immunodeficiency seemed to be irrelevant for supporting xeno-ectopic spermatogenesis. Our results confirmed that tubular reconstitution is applicable to porcine testicular cells. This method as well as the grafting method would be useful for studying spermatogenesis in different kinds of animals.

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The Whole Meiotic Process Can Occur in Vitro in Untransformed Rat Spermatogenic Cells

Cited by 86 publications

References 26 publications

Quantification of stem cell factor mRNA levels in the rat testis: usefulness of clusterin mRNA as a marker of the amount of mRNA of sertoli cell origin in post pubertal rats

Quantification of stem cell factor mRNA levels in the rat testis: usefulness of clusterin mRNA as a marker of the amount of mRNA of sertoli cell origin in post pubertal rats

The insulin sensitiser metformin regulates chicken Sertoli and germ cell populations

Ectopic porcine spermatogenesis in murine subcutis: tissue grafting versus cell-injection methods

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