We cloned the full-length cDNA of ZP2 from Carassius auratus var. Pingxiangnensis (CaP_ZP2) and identified a cluster of three ZP genes through its DNA walker. These three genes, CaP_ZP3.1, CaP_ZP2 and CaP_ZP3.2 were located within a 10,855bp region and each comprised of eight exons spanning 1348bp, 1638bp and 1348bp, respectively. Protein bands of egg membrane between 40 and 70kDa were in concordance with the deduced amino acid of these three CaP_ZP genes cDNA and with their molecular mass. This is the first report that two CaP_ZP3 genes were separated by CaP_ZP2 gene. A novel sequence of 1097bp, located between CaP_ZP2 and CaP_ZP3.2, was inserted into the modified pAcGFP1-1 vector in the forward and reverse directions. Results showed that individual sequence served as promoters utilizing common regulatory elements in the forward and reverse directions for both CaP_ZP2 and CaP_ZP3.2 gene expressions. In situ hybridization against CaP_ZP2 confirmed that a strong positive signal was detected in the early development oocytes. Similarly, real-time PCR results also showed that CaP_ZP2 transcription increased mainly in a 4–8month ovary, but was decreased dramatically in a 9–12month ovary.