Spermatogenesis in the dog

Foote, R.H.; Swierstra, E. E.; Hunt, W. L.

doi:10.1002/ar.1091730309

Cited by 94 publications

(49 citation statements)

References 16 publications

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“…To answer this question, we quantitated the corresponding type A and type B spermatognia. The number of type B spermatogonia at stage 7 in the control group was almost identical to that reported by Foote et al [22]. The ratio of type B to type A spermatogonia @/A) in both FRP-treated and control groups rapidly increased at stages 6-7 and decreased during stages 7 and 8.…”

Section: K Fujimori Et Alsupporting

confidence: 87%

Inhibition of Canine Spermatogonial Mitosis with Follicle Regulatory Protein

Fujimori

Montz

Nakamura

et al. 1986

Archives of Andrology

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Evidence was found that the Graafian follicle produces and secretes a hormonelike protein, referred to as follicle regulatory protein (FRP), which affects the responsivity of other follicles to gonadotropin stimulation. Since a similar material was identified in homogenates of bull testes, we evaluated the effects of FRP on the histology of seminiferous epithelium by its systemic injection into normal dogs. Mongrel dogs were injected IM with 5 mg of FRP for 17 consecutive days. The seminiferous epithelium was evaluated by light microscopy and divided into eight stages according to Foote. The relative frequency of stage 4 was significantly less in the FRP-treated than in the control group, but that of stage 7 was significantly greater in the FRP-treated group. The ratios of type B/type A spennatogonia for control and FRP-treated groups for stages 6-8 were 1.5, 5.8, 2.4, and 1.6, 4.3, 1.6, respectively. The tubular diameters of stages 6 and 7 were significantly different between the two groups. The numbers of tubules containing spermatogonial divisions were significantly decreased at stages 2 + 3 and stages 6+7 in the FRP-treated group. A clear decrease in the number of tubule profiles with spermatogonial divisions was present at stages 6 and 7 in the FRP-treated testis. Taken together, these findings suggest that FRP inhibits spermatogonial transformation of type A into type B.

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Section: K Fujimori Et Alsupporting

confidence: 87%

Inhibition of Canine Spermatogonial Mitosis with Follicle Regulatory Protein

Fujimori

Montz

Nakamura

et al. 1986

Archives of Andrology

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“…The second way to divide the seminiferous epithelial cycle uses cellular associations of defined composition in conjunction with variations in shape and localization of spermatids. This method has been established for a number of domestic animals (CLERMONT, 1972;FOOTE et al, 1972;SWIERSTRA et al, 1974;EKSTEDT et al, 1986), leads to a restricted number of stages (mostly 8), and is especially well suited for comparative and quantitative studies. According to this latter method the spermatogenic cycle in the buffalo seminiferous epithelium is divided into 8 stages with accomplished spermiation as the demarcation between the two cycles, as has been proposed by EKSTEDT et al (1986) for the bovine seminiferous epithelium.…”

Section: Methodsmentioning

confidence: 99%

Quantitative Aspects of Water Buffalo (Bubalus bubalis) Spermatogenesis.

Pawar

Wrobel

1991

Archives of Histology and Cytology

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“…of spermatogenesis by the increased T volume in the testes. The duration of spermatogenesis in the dog has been reported to be 54.4 days [5], and the duration of transit of sperm through the epididymis in many mammalian species is 8-14 days [14]. Therefore it is assumed that a small number of sperm had already been presented in a few seminiferous tubules before AI treatment.…”

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confidence: 99%

Therapeutic Effect of Aromatase Inhibitor in Two Azoospermic Dogs with High Plasma Estradiol-17β Levels

Kawakami

Taguchi

Hirano

et al. 2003

The Journal of Veterinary Medical Science

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ABSTRACT. Two azoospermic dogs with high plasma estradiol-17β (E 2 ) levels were subcutaneously injected with an aromatase inhibitor (AI), 4-androstene-4-ol-3,17-dione, 2 mg every other day for 4 weeks. Before the AI treatment the plasma E 2 levels of the two dogs (21 and 22 pg/ml, respectively) were higher than those of 2 normal dogs (8.1 and 12.3 pg/ml), and they fell to 11-17 pg/ml between 1 and 4 weeks after the start of AI treatment. The plasma testosterone levels after the start of AI treatment had increased to 2.1-3.1 ng/ ml. A small number of sperm were detected in the semen of the two dogs between 3 and 6 weeks after the start of AI treatment. Th ese results indicate that the testicular function of infertile dogs with high plasma E 2 levels can be temporarily improved by AI therapy. KEY WORDS: aromatase inhibitor, azoospermia, canine.J. Vet. Med. Sci. 65(12): 1343-1345, 2003 A portion of the testosterone (T) produced by the testis is converted to estradiol-17β (E 2 ) by aromatase enzyme activity [11]. In the testes of many species [2,17], including dogs [3], the E 2 -secreting cells are the Sertoli cells and/or the Leydig cells [13,20]. In men [6,19] abnormally increased testicular E 2 production causes spermatogenic dysfunction, and long-term E 2 administration has been shown to inhibit spermatogenesis in dogs [8,15]. Aromatase inhibitor (AI) blocks the aromatization of androgen to E 2 by inhibiting aromatase enzyme activity [1,18], and AI has been reported to be effective in treating spermatogenic dysfunction in men with high plasma E 2 levels [4]. In the present study, two azoospermic dogs with abnormally increased plasma E 2 levels were treated with AI to improve poor semen quality. Plasma E 2 levels after administration of follicle stimulating hormone extracted from porcine pituitary gland (FSH-P) were measured to investigate the main E 2 -secretory cells in canine testes.The two azoospermic dogs used to assess the effects of AI treatment were a Miniature Poodle (Dog 1) and a Beagle (Dog 2), aged 5 and 2 years, respectively. Dog 1 was owned by a breeder, and Dog 2 was cared for in our university. None of a few bitches mated with either of the two male dogs had conceived. Four semen specimens were collected by digital manipulation with a teaser bitch at one-week intervals. Each specimen was examine for total semen volume, total number of sperm, and morphologically abnormal sperm by the methods described previously [9]. As no sperm had been found in the semen of either Dog 1 or Dog 2 (Table 1), both of them were diagnosed as having azoospermia. Although the two azoospermic dogs were treated with 3 intramuscular injections of 1000 IU hCG per head at one-week intervals, their semen quality had failed to improve. Peripheral blood samples were collected from the two azoospermic dogs at the same time as the semen collections. Plasma E 2 and T levels were measured by the radioimmunoassay described previously [8]. The plasma E 2 levels of the two dogs (21 and 22 pg/ml, respectively) were higher than those o...

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Spermatogenesis in the dog

Cited by 94 publications

References 16 publications

Inhibition of Canine Spermatogonial Mitosis with Follicle Regulatory Protein

Inhibition of Canine Spermatogonial Mitosis with Follicle Regulatory Protein

Quantitative Aspects of Water Buffalo (Bubalus bubalis) Spermatogenesis.

Therapeutic Effect of Aromatase Inhibitor in Two Azoospermic Dogs with High Plasma Estradiol-17β Levels

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Spermatogenesis in the dog

Cited by 94 publications

References 16 publications

Inhibition of Canine Spermatogonial Mitosis with Follicle Regulatory Protein

Inhibition of Canine Spermatogonial Mitosis with Follicle Regulatory Protein

Quantitative Aspects of Water Buffalo (Bubalus bubalis) Spermatogenesis.

Therapeutic Effect of Aromatase Inhibitor in Two Azoospermic Dogs with High Plasma Estradiol-17&beta; Levels

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Therapeutic Effect of Aromatase Inhibitor in Two Azoospermic Dogs with High Plasma Estradiol-17β Levels