长链非编码核糖核酸肺腺癌转移相关转录本1和核旁斑组装转录本1在低氧预适应小鼠海马神经保护中的作用研究OA北大核心CSTPCD
The role of lncRNA MALAT1 and NEAT1 in neuroprotection of hypoxia preconditioning mouse hippocampus cell
目的 探索长链非编码核糖核酸(lncRNA)肺腺癌转移相关转录本1(MALAT1)和核旁斑组装转录本1(NEAT1)在低氧预适应(HPC)小鼠海马细胞中的表达及其与神经保护的关系.方法 (1)将36只雄性美国癌症研究所(ICR)小鼠按照随机数字表法完全随机分为3组:对照组、低氧组和低氧预处理组,每组12只.对照组小鼠不进行低氧暴露,低氧组小鼠低氧暴露1次,低氧预处理组小鼠低氧暴露4次.低氧处理结束后立即将所有小鼠脱颈椎处死并分离海马组织分组保存.(2)将HT22细胞培养于含10%胎牛血清和100 U/ml青霉素-链霉素的培养基,细胞汇合率大于90%时将其转移至24孔板中培养后分2批进行处理.通过转染试剂将6 pmol的乱序小干扰核糖核酸(siRNA)、MALAT1 siRNA(siMALAT1)、siNEAT1、siMALAT1+siNEAT1 分别一一对应转染至第一批HT22细胞的阴性对照组、siMALAT1组、siNEAT1组、siMALAT1+siNEAT1组细胞中,空白组不做任何处理;然后在正常条件下(5%CO2和95%空气)培养48 h;第二批HT22细胞中,利用转染试剂分别将 6pmol 的乱序 siRNA、乱序 siRNA、siMALAT1、siMALAT1、siNEAT1、siNEAT1 分别一一对应转染至阴性对照组、阴性对照+氧糖剥夺-再灌注(OGD/R)组、siMALAT1组、siMALAT1+OGD/R组、siNEAT1组、siNEAT1+OGD/R组的HT22细胞中,转染后48 h将阴性对照组、siMALAT1组、siNEAT1组HT22细胞在正常条件下(5%CO2和95%空气)继续培养,将阴性对照+OGD/R组、siMALAT1+OGD/R组、siNEAT1+OGD/R组细胞进行OGD/R处理,即低氧条件下(1%O2+5%CO2+94%N2)暴露8 h,之后再进行正常条件下培养16h.(3)通过实时荧光定量聚合酶链反应(PCR)及蛋白免疫印迹法测定各组小鼠海马组织中MALAT1、NEAT1、N-甲基-D-天冬氨酸受体亚基2B(NR2B)信使核糖核酸(mRNA)、NR2B蛋白水平的相对表达量和各组HT22细胞转染处理后NR2B mRNA、NR2B蛋白水平的相对表达量及各组HT22细胞转染和OGD/R后的血影蛋白分解产物、活化半胱氨酸蛋白酶蛋白3的相对表达量,并计算各组HT22细胞存活率.结果 (1)3组小鼠海马中MALAT1(F=43.92)、NEAT1(F=506.40)、NR2B mRNA(F=50.64)及 NR2B 蛋白(F=41.24)的相对表达量差异均有统计学意义(均P<0.05).与对照组相比,低氧组MALAT1[(1.68±0.06)比(1.00±0.08)]、NR2B mRNA[(1.26±0.06)比(1.00±0.01)]及 NR2B 蛋白[(1.47±0.05)比(1.00±0.01)]的相对表达量均增加(均P<0.05),而NEAT1[(1.02±0.10)比(1.00±0.03)]的相对表达量组间差异无统计学意义(P>0.05),低氧预处理组中MALAT1[(1.12±0.13)比(1.00±0.08)]和NEAT1[(2.88±0.10)比(1.00±0.03)]的相对表达量增加;与低氧组比较,低氧预处理组NR2B mRNA[(0.54±0.07)比(1.26±0.06)]及 NR2B 蛋白[(1.17±0.07)比(1.47±0.05)]的相对表达量均降低(均 P<0.05).(2)5 组 HT22 细胞转染后 NR2B mRNA(F=36.92)及 NR2B 蛋白(F=56.98)的相对表达量差异均有统计学意义(均P<0.05).与阴性对照组相比,siMALAT1组[NR2B mRNA:(2.04±0.08)比(0.94±0.04),NR2B 蛋白:(1.72±0.13)比(0.93±0.02)]、siNEAT1 组[NR2B mRNA:(2.15±0.13)比(0.94±0.04),NR2B 蛋白:(1.87±0.46)比(0.93±0.02)]、siMALAT1+siNEAT1组[NR2B mRNA:(2.09±0.16)比(0.94±0.04),NR2B 蛋白:(2.07±0.30)比(0.93±0.02)]的 NR2B mRNA及NR2B蛋白的相对表达量均增加(均P<0.05).(3)6组HT22细胞转染及OGD/R处理后血影蛋白分解产物(145/150 kDa蛋白;F=12.43)、血影蛋白分解产物(120 kDa蛋白;F=7.15)、活化的半胱氨酸蛋白酶蛋白3蛋白(F=6.61)的相对表达量差异均有统计学意义(均P<0.05).与 siMALAT1 组比较,siMALAT1+OGD/R 组的 145/150kDa[(1.42±0.48)比(0.85±0.34)]、120 kDa[(1.33±0.37)比(0.52±0.19)]的血影蛋白分解产物及活化的半胱氨酸蛋白酶蛋白3蛋白[(2.43±0.35)比(1.15±0.24)]相对表达量均增加(均P<0.05);与阴性对照+OGD/R组比较,siMALAT1+OGD/R 组的 145/150kDa[(1.42±0.48)比(1.23±0.17)]、120 kDa[(1.33±0.37)比(0.80±0.21)]的血影蛋白分解产物及活化的半胱氨酸蛋白酶蛋白3蛋白[(2.43±0.35)比(1.46±0.39)]相对表达量均增加(均 P<0.05);与 siNEAT1 组比较,siNEAT1+OGD/R 组的 145/150 kDa[(1.28±0.44)比(0.87±0.32)]、120kDa[(0.81±0.36)比(0.63±0.16)]的血影蛋白分解产物及活化的半胱氨酸蛋白酶蛋白3蛋白[(1.51±0.45)比(1.01±0.27)]相对表达量均增加(均P<0.05).(4)6组HT22细胞存活率差异有统计学意义(F=5.54,P<0.05).与阴性对照组比较,siMALAT1 组、siNEAT1 组、siMALAT1+OGD/R 组及 siNEAT1+OGD/R 组 HT22 细胞存活率均降低[(0.65±0.40)、(0.76±0.35)、(0.24±0.17)、(0.23±0.16)比(0.84±0.04),均 P<0.05];与siMALAT1 组比较,siMALAT1+OGD/R 组细胞存活率降低[(0.24±0.17)比(0.65±0.40),P<0.05];与 siNEAT1 组比较,siNEAT1+OGD/R 组细胞存活率降低[(0.23±0.16)比(0.76±0.35),P<0.05].结论 HPC增加了小鼠海马组织中 MALAT1和NEAT1的表达,MALAT1和NEAT1可能通过影响NR2B的表达参与小鼠缺血缺氧后的神经保护作用.
Objective To explore the expression of long non-coding ribonucleic acid(lncRNA)metastasis-associated lung adenocarcinoma transcript 1(MALAT1)and nuclear paraspeckle assembly transcript 1(NEAT1)in the hippocampus and HT22 cells of hypoxia pre-acclimated(HPC)mice and their relationship with neuroprotection.Methods(1)Thirty-six male Institute of Cancer Research(ICR)mice were randomly divided into three groups according to the random number table method of complete randomization:the control group,the hypoxia group and the hypoxia preconditioning group,with 12mice in each group.Mice in the control group were not exposed to hypoxia,mice in the hypoxia group were exposed to hypoxia once,and mice in the hypoxia preconditioning group were exposed to hypoxia four times.Immediately after the end of hypoxia treatment,all mice were decapitated and killed and hippocampal tissues were isolated and preserved in groups.(2)HT22 cells were cultured in medium containing 10%foetal bovine serum and 100 U/ml penicillin-streptomycin.When cell confluence was greater than 90%,they were transferred to 24-well plates for culture and then processed in 2 batches.6 pmol disordered small interfering RNA(siRNA),MALAT1 siRNA(siMALAT1),NEAT1 siRNA(siNEAT1),siMALAT1+siNEAT1 were transfected into the negative control group,siMALAT1 group,siNEAT1 group,and siMALAT1+siNEAT1 group of the first batch of HT22 cells one by one by transfection reagent,and the blank group did not have any treatment;then they were cultured under normal conditions(5%CO2 and 95%air)for 48 h.In the second batch of HT22 cells,6 pmol of disordered siRNA,disordered siRNA,siMALAT1,siMALAT1,siNEAT1 and siNEAT1 were transfected one by one correspondingly to the negative control group and the negative control+oxygen-glucose deprived/reoxygen(OGD/R)group,siMALAT1 group,siMALAT1+OGD/R,siNEAT1 group,siNEAT1+OGD/R group.48 h after transfection,HT22 cells of negative control group,siMALAT1 group and siNEAT1 group were cultured under normal conditions(5%CO2 and 95%air),and the cells of negative control+OGD/R group,siMALAT1+OGD/R group and siNEAT1+OGD/R group were treated with OGD/R.That is,under low oxygen conditions(1%O2+5%CO2+94%N2)exposure for 8 h,and then culture under normal conditions for 16 h.(3)The real-time fluorescence quantitative polymerase chain reaction(PCR)and Western blot was used to determine the expression of MALAT1,NEAT1,N-methyl-D-aspartate receptor subunit 2B(NR2B)messenger RNA(mRNA)and NR2B protein in the hippocampus of mice,the relative expression levels of NR2B mRNA and NR2B protein after transfection of HT22 cells in each group,and the relative expression levels of haemoglobin breakdown products and activated cysteine protease protein 3 after transfection and OGD/R of HT22 cells in each group.The survival rate of HT22 cells in each group was calculated.Results(1)The differences in relative expression of MALAT1(F=43.92),NEAT1(F=506.4),NR2B mRNA(F=50.64)and NR2B protein(F=41.24)in the hippocampus of mice in the three groups were statistically significant(all P<0.05).The relative expression of MALAT1([1.68±0.06]vs.[1.00±0.08]),NR2B mRNA([1.26±0.06]vs.[1.00±0.01]),and NR2B protein([1.47±0.05]vs.[1.00±0.01])was increased in the hypoxia group as compared to the control group(all P<0.05),whereas the relative expression of NEAT1([1.02±0.10]vs.[1.00±0.03])were not statistically significant(P>0.05),and the relative expression of MALAT1([1.12±0.13]vs.[1.00±0.08])and NEAT1([2.88±0.10]vs.[1.00±0.03])were increased in hypoxic preconditioned group.Compared with hypoxia group,the relative expression of NR2B mRNA([0.54±0.07]vs.[1.26±0.06])and NR2B protein([1.17±0.07]vs.[1.47±0.05])were decreased(both P<0.05).(2)The differences in the relative expression of NR2B mRNA(F=36.92)and NR2B protein(F=56.98)after transfection of HT22 cells in the five groups were statistically significant(both P<0.05).Compared with the negative control group,siMALAT1 group(NR2B mRNA:[2.04±0.08]vs.[0.94±0.04],NR2B protein:[1.72±0.13]vs.[0.93±0.02]),siNEAT1 group(NR2B mRNA:[2.15±0.13]vs.[0.94±0.04],NR2B protein:[1.87±0.46]vs.[0.93±0.02]),siMALAT1+siNEAT1 group(NR2BmRNA:[2.09±0.16]vs.[0.94±0.04],NR2B protein:[2.07±0.30]vs.[0.93±0.02])showed the relative NR2B mRNA and NR2B protein expression were increased(all P<0.05).(3)Differences in relative expression of haematopoietin breakdown product(145/150 kDa)protein(F=12.43),haematopoietin breakdown product(120 kDa)protein(F=7.15),and activated cysteamine protease protein 3 protein(F=6.61)were statistically significant in the 6 groups of HT22 cells transfected and treated with OGD/R(all P<0.05).Compared with the siMALAT1 group,the siMALAT1+OGD/R group had 145/150kDa([1.42±0.48]vs.[0.85±0.34]),120 kDa([1.33±0.37]vs.[0.52±0.19])haematopoietin catabolism products and activated cysteamine protease protein 3([2.43±0.35]vs.[1.15±0.24])relative expression increased(all P<0.05);compared with the negative control+OGD/R group,the siMALAT1+OGD/R group showed an increase in 145/150kDa([1.42±0.48]vs.[1.23±0.17]),120 kDa([1.33±0.37]vs.[0.80±0.21])relative expression of haematopoietin breakdown products and activated cysteamine protease protein 3([2.43±0.35]vs.[1.46±0.39])increased(all P<0.05);compared with the siNEAT1 group,the siNEAT1+OGD/R group had a higher expression of 145/150 kDa([1.28±0.44]vs.[0.87±0.32]),120 kDa([0.81±0.36]vs.[0.63±0.16])relative expression of haematopoietic proteolytic products and activated cysteamine protease protein 3([1.51±0.45]vs.[1.01±0.27])increased(all P<0.05).(4)The difference in HT22 cell survival rate among the 6 groups was statistically significant(F=5.54,P<0.05).Compared with the negative control group,HT22 cell survival was decreased in the siMALAT1,siNEAT1,siMALAT1+OGD/R and siNEAT1+OGD/R groups([0.65±0.40],[0.76±0.35],[0.24±0.17],[0.23±0.16]vs.[0.84±0.04],all P<0.05);cell viability was reduced in the siMALAT1+OGD/R group compared with the siMALAT1 group([0.24±0.17]vs.[0.65±0.40],P<0.05);and cell viability was reduced in the siNEAT1+OGD/R group compared with the siNEAT1 group([0.23±0.16]vs.[0.76±0.35],P<0.05).Conclusion HPC increased the expression of MALAT1 and NEAT1 in the hippocampus of mice,and MALAT1 and NEAT1 may participate in the neuroprotective effect of mice after ischemia and hypoxia by affecting the expression of NR2B.
侯海东;闫磊;王丽平;杨静;桂玉成;杜永强;邵国
523660 广东省东莞市清溪医院神经外科内蒙古低氧适应转化医学重点实验室广东省深圳市龙岗区第三人民医院转化医学中心
低氧预处理长非编码RNAMALAT1NEAT1NR2B
Hypoxic preconditioningLong non-coding RNAMALAT1NEAT1NR2B
《中国脑血管病杂志》 2024 (008)
525-536 / 12
国家自然科学基金(82060337);深圳市科技计划项目基础研究面上项目(JCYJ20220531092412028、JCYJ20230807121306012);深圳市龙岗区医疗卫生科技计划项目(LGKCYLWS2021000033、LGKCYLWS2023025)
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