The identification molecular marker relevant to male sterility is very important in breeding program. Precise prediction of male sterility at seedling stage can certainly shorten the breeding protocol and schedule. In this study, CMSP1 and CMSP2 primer sets were designed according to Capsicum annuum cytoplasmic male sterilityassociated protein gene (DQ116040, ORF456). A 402bp DNA fragment specific to pepper male-sterile cytoplasm could be successfully amplified from cDNA of flower buds(3-5mm in length)of the TSIPS male-sterile pepper lines by CMSP1 primers. Moreover, such specific PCR product could be amplified by CMSP1 from other male-sterile pepper lines, including lines developed from AVRDC-TWVC, ARI, and TSIPS. Using CMSP2 primer set, two additional reproductive PCR products(1200bp, 1500bp)besides the expected 350bp fragment were amplified and cloned from the male-sterile lines. The result of sequence alignment indicated that such clones were composed of sequences of coxⅡ gene (DQ126683.1；Cap. coxⅡ ) and cytoplasmic male sterilityassociated protein gene. Interestingly, although their sequences contained no primer sequences, these fragments were stably produced. Besides CMSP1 and CMSP2, ATP-1, ATP-2 and ATP-3 primer sets designed according to pepper atp6-2 gene sequence could also produce reliable marker specific to pepper cytoplasmic male sterility lines. Moreover, the residual mitochondrial DNA in DNA extracts of seedling leaves was adequate for PCR amplification by these primer sets, which means the laborious mitochondria DNA extraction may not be necessary.