目的:构建跨膜蛋白超家族6成员2（Tm6sf2） E167K基因敲入小鼠模型。方法:构建同时表达针对小鼠Tm6sf2基因特定位点的单链向导RNA Cas9的质粒和携带Tm6sf2 E167K片段的Donor质粒，将上述2质粒一起注射入小鼠受精卵，通过PCR检测和测序验证得到F0代阳性小鼠。统计F2代中野生（Wt）、杂合和敲入（KI）3种基因型小鼠的存活数量。选取F2代同窝Wt和KI雄性小鼠（8只/组）给予普通饮食8周，每周记录小鼠的体质量，检测两种小鼠葡萄糖代谢和脂质代谢等指标。组间比较采用独立样本n t检验。n 结果:基因型检测和测序结果表明Tm6sf2 E167K基因敲入小鼠模型建立成功。KI小鼠不存在胚胎纯合致死的表型。哺乳期内KI小鼠较Wt小鼠的体质量升高，两组差异有统计学意义（n P 0.05). The Oil red O staining results showed that KI mice had more lipid accumulation in the centrilobular region of ??liver than Wt mice.n Conclusion:Tm6sf2 E167K gene knock-in mice were successfully constructed. Tm6sf2 E167K gene knock-in can cause abnormal glucose metabolism in mice and promote the occurrence of hepatic steatosis.