In Klebsiella pneumoniae CG43, deletion of pecS or pecM, which located in-between the type 1 and type 3 fimbriae gene clusters, had previously been shown to increase the expression of type 3 fimbriae major pilin MrkA. Here the deleting effect of pecS and pecM is further analyzed. The analysis of western blotting hybridization, mannose sensitive yeast agglutination, and biofilm formation activity revealed that either gene deletion increased the expression of type 3 fimbriae but had no apparent influence on type 1 fimbriae expression. Notably, the deleting effect of pecM on type 3 fimbriae was more apparent than that of pecS. Addition of urate was able to increase the MrkA expression and biofilm forming activity, however, deletion of the pecM had lost of the urate induced activity. This implied that the transmembrane domain of PecM may be involved in the transport or sensing uric acid for biofilm formation. Moreover, EMSA analysis indicated that the recombinant PecS was able to bind to the the putative pecO-containing promoters PmrkA, PpecS or PpecM. The following competitive assay suggests that uric acid is a ligand of the recombinant PecS to prevent from the binding to the pecO-containing DNA. Moreover, the promoter activity measurement revealed that the level of PpecS, PpecM, or PmrkA increased by the deletion of pecS. Taken together, these results suggest that PecM and PecS are able to negatively regulate the expression of type 3 fimbriae and PecS could also repress pecS and pecM expression at the transcriptional level. Finally, disc inhibition assay failed to detect either gene deleting effect on the bacterial response to paraquat treatment. The 2-hybrid analysis was also unable to demonstrate the interaction between PecS and PecM.