This study was conducted to establish a system of molecular marker-assisted selection through exploring RNAseq SSRs and constructing a preliminary linkage map for genetic analysis using the segregation population crossed between Chinese type, ‘Keumsull’ and Assamese type, ‘Ai37’. First, transcripts of flowers and young shoots collected from ‘Ai37’ were sequenced and compared to the transcript sequences of ‘Keumsull’. Then, 1,800 SSR motifs were mined, and 226 SSR primers were designed. These primers were validated for the presence of polymorphism with two parents and six progenies together, and then 96 primers were selected. After extensively applying to two parents and 66 hybrids of the F1 population, 87 primers showing apparent recognition for segregation of SSR markers were finally selected. Linkage analysis for SSR amplification and genotype segregation was performed using the JoinMap 4.0 program, and then a preliminary genetic map was constructed using MapChat 2.32 program. The preliminary genetic map consisted of 5 linkage groups with 14 SSR markers and had a total genetic distance of 167.0 cM with an average distance between the markers of 11.9 cM. The number of loci for the SSR markers located on the genetic map was 2 to 5 consisting of 1 to 4 alleles in a locus, and an average of 2 alleles per locus was identified. The results indicated that the development of RNAseq-based SSR markers and genetic analysis might be affected by the composition of RNA pool, parent genetic similarity, and segregation population size. A strategy for improving saturation and further studies are required in the future.