摘要目的 分析结核分枝杆菌katG基因2个不同区域的基因变异,并确定与INH耐药的相关性.方法 从痰液分离并鉴定结核分枝杆菌耐INH菌株53株,用PCR扩增katG基因的2个区域:区域1为第1位密码子至150位密码子,区域2为第227位密码子至470位密码子,并分别测序.结果 3株对INH耐药但2个区域都不发生突变.14株区域1存在突变,其中5株只在区域1存在突变,5株在区域1出现缺失突变,并呈现高度耐药.点突变是区域2的主要特点,特别是S315位密码子,60.4%(32/53)S315发生突变,最常见的是S315N(AGC→AAC)(18株);katG S315在高度INH耐药和低度INH耐药的结核分枝杆菌中突变率分别是84.4%(27/32)、15.6%(5/32),两组间差异有统计学意义(x2=30.25,P＜0.01).27株S315突变呈高度耐药,占S315突变菌株总数的84.4%,其余18株至少有一个非S315点突变的耐药株中高度耐药只有5株,占27.7%,两组间差异有统计学意义(x2=16.02,P＜0.01).对INH耐药的结核分枝杆菌区域2的突变发生率为84.9%.5株只在区域1存在突变,通过检测基因突变诊断INH耐药的检出率上升至94.3%.结论 S315突变发生率最高,突变类型和位置与耐药程度密切相关,分析区域1能使检出率提高9.4%.

abstractsObjective To analyze and compare the mutations in two different regions of the katG gene and study the relevance of Mycobacterium tuberculosis isoniazid-resistance and mutations in two different regions of the katG gene. Methods Fifty-three INH-resistant Mycobacterium tuberculosis strains isolated in cultures of sputum samples obtained from Zhejiang province were analyzed. PCR was used to amplify two regions of the katG gene (GenBank accession no. U06258) region 1 (from codon 1 to codon 150) and region 2 ( from codon 227 to codon 470) which were then sequenced in order to identify mutations. Results Three strains resistant to INH did not contain mutations in either region. Fourteen strains carried mutations in region 1. Among them 5 strains barbered deletions, and showed high-level resistance to isoniazid. Five strains had mutations only in region 1. Region 2 carried multiple point mutations, especially at codon 315, and there were S315 N ( AGC→AAC ) substitution in 18 of those cases. The frequency of mutations in the katG S315 of high-level INH-resistance isolates ( 84. 4%, 27/32) was significantly higher than those of low-level INH-resistance isolates( 15.6%, 5/32 ), there was statistically significant difference (x2 = 30. 25, P ＜ 0. 01 ).katG S315 mutations in high-level INH-resistance frequency (84. 4%, 27/32) was significantly higher than the other mutations of katG gene of high-level INH-resistance frequency (27. 7%, 5/18 ), there was significant difference (x2 = 16.02, P ＜ 0. 01 ). The analysis of region 2 allowed INH resistance to be diagnosed in 84. 9% of the strains. Five strains had mutations only in region 1 ,which allowed the proportion of INH-resistant strains identified to be increased to 94. 3%. Conclusions The number of mutations at codon 315 was high. Mutation type and location closely related with drug resistance and the analysis of region 1 resulted in a 9. 4% increase in the rate at which mutations were identified.