Role of TRPV1 channels during the acquisition of fertilizing ability in boar spermatozoa

When spermatozoa from specific segments of the epididymis were inseminated intra-tubally, ten hours before ovulation, virtually no ova were fertilized by sperm samples taken from the regions proximal to the middle of the corpus epididymidis. Sperm from the caput epididymidis and the proximal half of

Human spermatozoa freed from seminal plasma using a discontinuous Percoll gradient procedure were incubated overnight in modified Tyrode's media containing either CaClz (CA medium) or with SrCl2 instead of CaC12 (SR medium). The following morning these spermatozoa were washed by centrifugation, resu

## Abstract The effects, of testosterone, 17βT‐hydroxy‐5α‐androstane‐3‐one (5α‐dihydrotestosterone; 5α‐DHT), 5α‐androstane‐3α, 17βT‐diol (3α‐androstanediol; 3α‐diol) and 5α‐androstane‐3βT, 17βT‐diol (3βT‐androstanediol; 3βT‐diol) on the development of fertilizing ability by spermatozoa in the epidi

## Abstract A variety of treatment procedures was utilized to identify the origin and composition of the vesicles formed during the acrosome reaction of boar spermatozoa. Whether the acrosome reaction occurred spontaneously or was induced chemically the vesicles were hybrid vesicles composed of rou