In order to amplify the partial bcl-2 gene of goose,we designed a pair of primers according to the reported chicken bcl-2 gene sequence in the GenBank,and obtained the gene by reverse transcript-polymerase chain reaction(RT-PCR).Then the gene was cloned into pMD-18T vector and identified by PCR.The nucleotide and amino acid sequences of goose partial bcl-2 gene were compared with the counterpart sequences of chicken,and the nucleotide homology was 92.49%.This is the first report of bcl-2 partial nucleotide sequence of goose.
Inhibin a is one of the candidate genes that control the ovulation in poultry. To study the genetic effects of inhibin a on apoptosis and proliferation of goose granulosa cells cultured in vitro, two RNA interference (RNAi) expression vectors, psiRNA-INHal and psiRNA-INHα2, were constructed to knock down inhibin α gene expression. After 48 h of transfection, the efficiency of these two RNAi expression vectors was examined by fluorescence microscopy. Meanwhile, inhibin protein expression levels, apoptosis indexes (AI) and proliferation indexes (PI) of granulosa cells were analyzed by flow cytometry. In addition, the supernatants were collected to assay the concentrations of estrogen (E2) and progesterone (P) by radioimmunoassay. The results showed that the expression level of inhibin a in the RNAi group were decreased 30%--40% than those in the control groups (P 〈0.05) and the apoptosis indexes and proliferation indexes in the RNAi groups were significantly higher than those in the control groups (P 〈0.05). However, the E2 concentrations in the RNAi groups were lower than those in the control groups (P 〈0.05). These results indicate that inhibin a has antagonistic effect on granulosa cell apoptosis.
Based on published sequences for chicken Bcl-2,three siRNAs(small interfering RNA)were designed,and expression vectors were constructed and transfected into goose granulosa cells cultured in vitro.Bcl-2 protein,apoptosis and proliferation of granulosa cells,48 h after the transf ection,were analyzed by flow cytometry,and progesterone(P)secreted into the culture medium was measured by radioimmunoassay.In addition,apoptosis and Bcl-2 protein level were assessed in untreated granulosa cells from the four largest preovulatory follicles(F1F4),the smallest preovulatory follicles(SPF),small yellow follicles(SYF)and atretic follicles.The highest level of Bcl-2 protein was observed in granulosa cells from SPF,and levels in cells from healthy follicles were significantly higher than those of atretic follicles(P<0.05).Bcl-2 protein levels in cells subjected to RNAi were significantly lower than those of controls(P<0.05),while apoptosis indices(AI),proliferation indices(PI)and P secretion in the RNAi treatments were higher than those of controls(P<0.05).
