17 research outputs found

    Effects of 17a-methyltestosterone on seminal vesicle, development and semen release response in the African catfish, Clarias gariepinus

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    The effects of 17alpha-methyltestosterone on seminal vesicle development in the African catfish, Clarias gariepinus, were investigated in an attempt to improve semen collection from this species. Treatment of larvae with dietary 17alpha-methyltestosterone at 50 mg kg(-1) for days 12-33 or days 12-40 after hatching, or at 20 mg kg(-1) for days 12-26, 12-33, 12-40 or 12-47 after hatching inhibited the development of the seminal vesicle finger-like extensions in male catfish, but did not affect the sex ratio. The minimum effective dose and period of treatment to inhibit seminal vesicle development in all male catfish treated with 17alpha-methyltestosterone was 20 mg kg(-1) for days 12-40 after hatching. Male catfish from this treatment group developed normal testes that, in some cases, contained a few oocytes, which tended to disappear before sexual maturation. After sexual maturation, the semen release response was evaluated in males with incomplete seminal vesicles. Fluid with viable spermatozoa was obtained after two consecutive injections of carp pituitary suspension, from 10 of 19 males that had been fed 20 mg 17alpha-methyltestosterone kg(-1) for days 12-40 or days 12-47 after hatching, but from only 4 of 15 males that did not receive any dietary steroid. Intratesticular semen quality was not affected by 17alpha-methyltestosterone treatment. The results of this study demonstrate that the absence of seminal vesicle extensions induced by treatment with 17alpha-methyltestosterone facilitated the collection of semen by stripping from this species of fish

    Effects of oxytocin on semen release response in African catfish (Clarias gariepinus)

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    In silurid fishes, semen collection is practically impossible, even after hormonal stimulation. Instead, males are killed and testes macerated to obtain sperm. To understand the endocrine control of semen release in catfishes, we investigated the role of smooth muscle contractors in semen release and semen quality of African catfish (Clarias gariepinus). In in vitro experiments, testis slices were incubated with oxytocin (1 and 10 IU), isotocin (2 and 20 ug), vasopressin (0.2 and 2 ug), epinephrine (1 and 10 ug), PGF2alpha (1 and 10 ug), purified Clarias LH (300 ng) and partly purified Clarias pituitary extract (containing 300 ng LH). Only oxytocin increased sperm concentration of the medium (assessed by optical density measurements) compared to control incubations. Oxytocin was then tested in vivo in two groups of fish: normal males, and males that had been treated with 17alpha-methyltestosterone during larval stages to inhibit seminal vesicle development (NIT males). Both groups of fish received two doses of carp pituitary suspension (8 and 10 mg/kg, respectively i.m.) with or without subsequent oxytocin treatment (5 IU/kg i.v.; cPS-OT treatment and cPS treatment, respectively). There was no effect of oxytocin on the number of strippable males. Of cPS and cPS-OT treated fish, 87% MT males and 60% normal males were, strippable. The stripped semen volume was low in both groups but MT males produced higher (P <0.001) hatching rates (63.1%) than did normal males (2.1%). (C) 2002 Elsevier Science Inc. All rights reserved

    Sucesso do resfriamento e congelamento de sĂȘmen de pirapitinga Brycon nattereri Sucess of cooling and freezing of pirapitinga (Brycon nattereri) semen

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    Avaliaram-se protocolos de resfriamento e de criopreservação do sĂȘmen de pirapitinga (Brycon nattereri) utilizando-se sĂȘmen diluĂ­do em NaCl 154mM, NaCl 200mM, Saad e BTSÂź e resfriado por sete dias. Cinco diluidores (glicose 277mM, NaCl 154mM, NaCl 200mM, Saad e BTSÂź) foram combinados com dois crioprotetores (DMSO - dimetilsulfĂłxido e metilglicol) e usados como meio de congelamento. O sĂȘmen diluĂ­do em cada meio foi envasado (palhetas de 0,5ml) e congelado, e a motilidade espermĂĄtica avaliada apĂłs o descongelamento (60&deg;C, 8seg). O sĂȘmen foi novamente congelado em palhetas com diferentes volumes (0,25 e 0,5ml) e descongelados em banho-maria em duas temperaturas (50&deg; e 60&deg;C). As maiores motilidades (48%) foram observadas no sĂȘmen diluĂ­do em BTSÂź e resfriado por sete dias. Motilidade espermĂĄtica acima de 68% foram observadas no sĂȘmen congelado em NaCl 154mM-metilglicol, BTSÂź-metilglicol, NaCl 200mM-DMSO e Saad-DMSO. NĂŁo houve diferença entre os volumes de palheta nem entre as temperaturas de descongelamento quanto a motilidade espermĂĄtica. Assim, o sĂȘmen de pirapitinga mantĂ©m altas taxas de motilidade quando resfriado em BTSÂź por atĂ© sete dias ou congelado em NaCl 154mM-metilglicol, BTSÂź-metilglicol, NaCl 200mM-DMSO e Saad-DMSO.Cooling and freezing protocols of pirapitinga (Brycon nattereri) semen were evaluated using semen diluted in 154mM NaCl, 200mM NaCl, Saad or BTS&trade;, and cooled for seven days. Sperm motility was daily evaluated. Five extenders (277mM glucose, 154mM NaCl, 200mM NaCl, Saad and BTS&trade;) were combined with two cryoprotectants (DMSO - dimethyl sulphoxide and methylglycol) to produce 10 cryosolutions. Semen was diluted in each cryosolutions, aspirated into 0.5ml straws and frozen. Sperm motility was evaluated after thawing (60&deg;C, 8 sec). Then, semen was frozen in straws with different volumes (0.25 and 0.5ml), and thawed under different water-bath temperatures (50&deg; and 60&deg;C). Higher sperm motility (48%) was observed when semen was cooled in BTS&trade; for seven days. Post-thawing sperm motility above 68% was observed when semen was frozen in 154mM NaCl-methylglycol, BTS&trade;-methylglycol, 200mM NaCl-DMSO or Saad-DMSO. There was no difference on sperm motility when semen was frozen in 0.25 or 0.5ml straws and thawed in 50&deg; or 60&deg;C water-bath. Thus, pirapitinga semen can be successfully cooled in BTS&trade; for seven days or frozen in 154 mM NaCl-methylglycol, BTS&trade;- methylglycol, 200mM NaCl-DMSO and Saad-DMSO
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