Literature DB >> 10022769

A rapid method of Sertoli cell isolation by DSA lectin, allowing mitotic analyses.

S Scarpino1, A R Morena, C Petersen, B Fröysa, O Söder, C Boitani.   

Abstract

We have developed a rapid and convenient method of Sertoli cell preparation for studying the growth kinetics of these cells in in vitro culture. Datura Stramonium agglutinin (DSA)-coated dishes were used to rapidly purify single Sertoli cells from immature rat testis. We have monitored by immunohistochemical markers the degree of contamination of our Sertoli cell preparation by other cell types. The cell preparation is essentially free of germ cells and interstitial cells and contains a minimal percentage of myoid cells. Sertoli cells isolated with this method retain functional activities such as the FSH responsiveness in terms of cAMP production. In addition, we have studied the proliferative activity of Sertoli cells isolated by lectin binding from rats of different ages. Sertoli cells exhibited a characteristic pattern of proliferation which was a function of the donor animal age. The proliferative activity of isolated Sertoli cells decreased with age, being much higher in 3 day-old rats than in older animals. A similar pattern was observed when the mitotic activity of Sertoli cells in response to mitogens present in the testicular extracts from 5 day-old rats was evaluated. The method described here reduces or eliminates many of the drawbacks of the conventional procedures used to isolate Sertoli cells, thus providing a useful tool in studies of growth kinetics and regulation of cell proliferation in vitro.

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Year:  1998        PMID: 10022769     DOI: 10.1016/s0303-7207(98)00190-7

Source DB:  PubMed          Journal:  Mol Cell Endocrinol        ISSN: 0303-7207            Impact factor:   4.102


  20 in total

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Journal:  J Assist Reprod Genet       Date:  2011-12-11       Impact factor: 3.412

2.  Effects of different Sertoli cell types on the maintenance of adult spermatogonial stem cells in vitro.

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Journal:  In Vitro Cell Dev Biol Anim       Date:  2017-07-11       Impact factor: 2.416

3.  In vitro culture and morphological characterization of prepubertal buffalo (Bubalus bubalis) putative spermatogonial stem cell.

Authors:  S Kala; R Kaushik; K P Singh; P H Kadam; M K Singh; R S Manik; S K Singla; P Palta; M S Chauhan
Journal:  J Assist Reprod Genet       Date:  2012-11-15       Impact factor: 3.412

4.  Starvation is more efficient than the washing technique for purification of rat Sertoli cells.

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Journal:  In Vitro Cell Dev Biol Anim       Date:  2014-05-02       Impact factor: 2.416

5.  Isolation of Sertoli Cells and Peritubular Cells from Rat Testes.

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Journal:  J Vis Exp       Date:  2016-02-08       Impact factor: 1.355

6.  Undifferentiated spermatogonia regulate Cyp26b1 expression through NOTCH signaling and drive germ cell differentiation.

Authors:  Parag A Parekh; Thomas X Garcia; Reham Waheeb; Vivek Jain; Pooja Gandhi; Marvin L Meistrich; Gunapala Shetty; Marie-Claude Hofmann
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7.  Utp14b: a unique retrogene within a gene that has acquired multiple promoters and a specific function in spermatogenesis.

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Review 8.  Characterization of rodent Sertoli cell primary cultures.

Authors:  Helena D Zomer; Prabhakara P Reddi
Journal:  Mol Reprod Dev       Date:  2020-08-02       Impact factor: 2.609

9.  Efficiency of adult mouse spermatogonial stem cell colony formation under several culture conditions.

Authors:  M Koruji; M Movahedin; S J Mowla; H Gourabi; A J Arfaee
Journal:  In Vitro Cell Dev Biol Anim       Date:  2009-02-17       Impact factor: 2.416

10.  Direct transdifferentiation of stem/progenitor spermatogonia into reproductive and nonreproductive tissues of all germ layers.

Authors:  Liz Simon; Gail C Ekman; Natalia Kostereva; Zhen Zhang; Rex A Hess; Marie-Claude Hofmann; Paul S Cooke
Journal:  Stem Cells       Date:  2009-07       Impact factor: 6.277

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