Bacterial tyrosine kinases have been recently unified in a new enzyme family because of the similar structural and functional features with their eukaryotic counterparts. Via an in vitro phosphorylation assay, the protein-tyrosine kinase Wzc of Klebsiella pneumoniae CG43 was shown capable of phosphorylating the capsular polysaccharide biosynthesis operon cps gene products 6-phosphogluconate dehydrogenase (Gnd), GDP-mannose phosphorylase (ManC) and phosphomannomutase (ManB) and the phosphorylation leading to increase of the enzymatic activities. In this study, we generate CG43S3Δgnd, CG43S3ΔmanC and CG43S3ΔmanB mutants and the phenotypes analyzed and compared. The analysis revealed that deletion of manC or manB decreased the glucuronic acid production but increased the biofilm formation. Several of the ManB tyrosine residues were then selected for site directed mutagensis in order to determine which is the one that subjected to Wzc phosphorylation and if the phosphorylation influences the enzymztic activity. The subsequent complementation analysis revealed that the manB deleting effect could be complemented by introducing into the mutant with the ManB expression plasmid pRK415-manB or the plasmid pRK415-manBY26F and pRK415-manBY341F which carrying a point mutation of ManB.Whereas the bacteria CG43S3ΔmanB carrying pRK415-manBY10F exhibited a partially restored phenotype implying the phosphorylation on tyrosine residue 10 of ManB was critical for the enzymatic activity. In addition, the ManB activity was decreased in the bacteria CG43S3ΔmanB [pETQ33-manBY10F] or CG43S3ΔmanB [pETQ33-manBY341F] by comparing to that in CG43S3ΔmanB [pETQ33-manB ] or CG43S3ΔmanB [pETQ33- manBY26F]. These recombinant plasmids were then overexpressed in E. coli BL21[DE3] and the recombinant proteins purified. The circular dichroism spectra analysis of the purified proteins revealed that the site directed mutation had no effect on the secondary structure. Finally, the in virto phosphorylation assay showed that the monoclonal antibody and Pro-Q Diamond were able to detect the ManB phosphorylation form and ManB phosphorylation slightly enhanced the enzymatic activity. In addition, the S98 was found to be a critical phosphorylation residue which is required for the enzyme activity. However,the serine phosphorylation was not afftected by the deletion of wzc or stk.