Objective: To knock out the entire Luxs gene of Streptococcus mutans(S.mutans) UA159 strain via homologous recombination and construct a Luxs-deleted mutant strain of S. mutans. To study the difference between the acid resistance of S. mutans Ingbritt C international standard strain and the acid resistance of LuxS mutant strain. Methods: Two DNA fragments locating in the upper and downstream of Luxs gene were amplified and a erythromycin resistance gene of PJT10 between them were engineered into PUC19 plasmid for constructing the recombination plasmid pUCluxKO. Electrotransformation of S.mutans cells with pUCluxKO-mutant resulted in isolation of erythromycin resistant S. mutans transformants, which was identified by polymerase chain reaction, V.harveyi BB170 luminescence bioassay and sequencing analysis. Solutions of S. mutans standard strain and LuxS mutant strain with same density were made and cultured at pH 3.5 to 7.0 BHI liquid for the same period.Terminal growth situation was compared.Firstly acidized in pH 5.5 BHI liquid,the two strains were cultured at pH 3.0 BHI liquid. The acid tolerance responses of the two strains were compared.Results:Restriction endonuclease analyses showed that pUCluxKO-mutant vector had been successfully recombined. The Luxs-deleted status of S.mutans mutants was confirmed by PCR with primers which were specific for the genes of Luxs and Erythromycin resistance. S.mutans mutant can not induce bioluminescence, indiating the mutant had been successfully recombined. After twenty generations of culture, the constructed Chinese S.mutans mutants were confirmed to be stable. Significant difference of aciduricity was observed between S.mutans standard strain and LuxS mutant strain.The acid resistance of standard strain was stronger than that of LuxS mutant strain.The two strains both displayed the capability of acid tolerance responses. Conclusion:The S.mutans gene allelic exchange plasmid is constructed correctively and a Luxs-negative mutants of S.mutans is constructed, which can help to further study the role of Luxs in the pathogenesis of S.mutans. LuxS mutant strain is more sensitive to acid inactivation,but the capability of acid tolerance responses exist still. Objective: To knock out the entire Luxs gene of Streptococcus mutans (S. mutans) UA159 strain via homologous recombination and construct a Luxs-deleted mutant strain of S. mutans. To study the difference between the acid resistance of S. mutans Ingbritt C international Standard strain and the acid resistance of LuxS mutant strain. Two DNA fragments locating in the upper and downstream of Luxs gene were amplified and a erythromycin resistance gene of PJT10 between them were engineered into PUC19 plasmid for constructing the recombination plasmid pUCluxKO. Electrotransformation of S. mutans cells with pUCluxKO-mutant resulted in isolation of erythromycin resistant S. mutans transformants, which was identified by polymerase chain reaction, V. harveyi BB170 luminescence bioassay and sequencing analysis. Solutions of S. mutans standard strain and LuxS mutant strain with same density were made and cultured at pH 3.5 to 7.0 BHI liquid for the same period. Terminal growth situation was com The acid tolerance responses of the two strains were compared. Results: Restriction endonuclease analysis showed showed pUCluxKO-mutant vector had been successfully recombined. The Luxs -deleted status of S. mutans was identified by PCR with primers which were specific for the genes of Luxs and Erythromycin resistance. S. mutans mutant can not induce bioluminescence, indiating the mutant had been successfully recombined. After twenty generations of culture, the constructed Chinese S. mutans mutants were confirmed to be stable. Significant difference of aciduricity was observed between S. mutans standard strain and LuxS mutant strain. acid resistance of standard strain was stronger than that of LuxS mutant strain. capability of acid tolerance responses. Conclusion: The S.mutans gene allelic exchange plasmid is constructed correctively and a Luxs-negative mutants of S.mutans is constructed, which can help to further study the role of Luxs in the pathogenesis of S.mutans. LuxS mutant strain is more sensitive to acid inactivation, but the capability of acid tolerance responses exist still.