Analysis of SMOC2 gene variants in familial and nonfamilial primary open angle glaucoma Pakistani patients

AIM:To find out the association of secreted protein acidic and rich in cysteine(SPARC)-related modular calcium binding 2(SMOC2)gene variants rs2255680 and rs13208776 with genotypic and phenotypic characteristics in both familial and non-familial primary open angle glaucoma(POAG)patients.METHODS:A total of 212 POAG patients,comprising 124 familial and 88 non-familial,were enrolled.For genotyping the SMOC2 variant rs2255680,amplification refractory mutation system(ARMS)-polymerase chain reaction(PCR)method and PCR-restriction fragment length polymorphism(PCR-RFLP)were utilized for analyzing rs13208776 variant.RESULTS:The mean age of familial POAG patients was 50.92±9.12y,with 78 males and 46 females.The mean age of non-familial POAG patients was 53.14±13.44y,with 52 males and 36 females.The SMOC2 gene variant rs13208776 showed the significant association with POAG between familial and non-familial groups.The homozygous G/G variant was frequent among non-familial(60.2%)whereas the heterozygous G/A variant was more frequent in familial POAG patients(46%).There were significant differences in G/A variant between familial and non-familial glaucoma patients,and the risk was decreased to 0.53-fold in non-familial glaucoma patients[odds ratio(OR):0.53;95%confidence interval(CI):0.29-0.94;P=0.033]in codominant model.The risk was further reduced to 0.49-fold(95%CI:0.28-0.86;P=0.012)in dominant model for non-familial patients.No significant association of SMOC2 gene variant rs2255680 between familial and non-familial glaucoma patients was found in our population.The haplotype analysis showed the decreased risk for TA[OR:0.48(95%CI:0.29-0.79);P=0.004]and an increased risk for TG[OR=2.28(95%CI:1.22-4.25);P=0.01]haplotypes.CONCLUSION:Current findings show significant association of SMOC2 gene variant rs13208776 with POAG between familial and non-familial Pakistani patients.

子宫内膜异位症患者子宫内膜组织中ID2、PRELP、SMOC2基因表达和临床意义

目的观察子宫内膜异位症患者子宫内膜组织中ID2、PRELP、SMOC2基因表达并分析其临床意义。方法选取2016年3月至2018年1月于郑州人民医院诊治的子宫内膜异位症患者102例为试验组,另选取同期本院收治的98例子宫肌瘤患者为对照组。qRT-PCR法检测两组子宫内膜组织中ID2、PRELP、SMOC2mRNA表达量,Western blot法检测子宫内膜组织中ID2、PRELP、SMOC2蛋白表达情况,观察患者临床指标并分析其与ID2、PRELP、SMOC2的相关性,制作受试者工作特征曲线(ROC),分析ID2、PRELP、SMOC2在子宫内膜异位症中的诊断效能,Logistic多元回归分析影响子宫内膜异位的相关因素。结果试验组患者子宫内膜组织中ID2、PRELP、SMOC2mRNA表达量及蛋白表达水平均高于对照组,差异有统计学意义(P<0.05);试验组患者子宫内膜组织中ID2与VEGF、IL-1β及CA125呈正相关(P<0.05),PRELP与VEGF、TNF-α及CA125呈正相关(P<0.05),SMOC2与IL-1β及CA125呈正相关(P<0.05);ROC曲线分析显示,子宫内膜组织中ID2、PRELP、SMOC2对子宫内膜异位症具有临床诊断价值;Logistic多元回归分析显示,子宫内膜组织中ID2、PRELP及SMOC2均为子宫内膜异位症患者的危险因素。结论子宫内膜异位症患者子宫内膜组织中ID2、PRELP、SMOC2基因表达升高,且与患者临床指标呈正相关,三者均参与病情发生进展过程,可作为临床诊断及监测子宫内膜异位症的重要指标。

甲状腺乳头状癌中SMOC2的表达与临床病理意义

目的探讨SMOC2在甲状腺乳头状癌(papillary thyroid carcinomas,PTC)中的表达及其与CK19、Galectin-3、MC和BRAF V600E联合辅助诊断的效能。方法采用生物信息技术学分析Gene Expression Omnibus数据库及The Cancer Genome Atlas数据库中SMOC2在PTC和良性甲状腺组织中的mRNA表达量差异;采用免疫组化EnVision法检测75例PTC和45例甲状腺乳头状增生(papillary thyroid hyperplasia,PTH)石蜡切片中SMOC2蛋白的表达,并分析其联合CK19、Galectin-3、MC和BRAF V600E进行辅助诊断的敏感度、特异性。结果生物信息学分析结果显示:SMOC2在PTC组织中的mRNA表达量显著低于良性甲状腺组织(P<0.05),且SMOC2对PTC诊断预测的曲线下面积(area under the curve,AUC)为0.910(P<0.001)。免疫组化结果显示:SMOC2在PTC中的表达显著低于PTH组织(P<0.001),且SMOC2对PTC诊断预测的AUC为0.898(P<0.001)。SMOC2与CK19、Galectin-3、MC和BRAF V600E五者联合辅助诊断PTC时的AUC为1.000(P<0.001),其余标志物相互组合时AUC值均低于1.000。结论SMOC2在PTC中的表达明显降低,可作为PTC诊断和鉴别诊断的重要标志物,与CK19、Galectin-3、MC和BRAF V600E五者联合辅助诊断PTC时可在一定程度上提高灵敏度和特异性。

Smoc2 potentiates proliferation of hepatocellular carcinoma cells via promotion of cell cycle progression

AIM To determine the influence of Smoc2 on hepatocellular carcinoma(HCC) cell proliferation and to find a possible new therapeutic target for preventing HCC progression.METHODS We detected expression of Smoc2 in HCC tissues and corresponding non-tumor liver(CNL) tissues using PCR, western blot, and immunohistochemistry methods. Subsequently, we down-regulated and upregulated Smoc2 expression using siR NA and lentivirus transfection assay, respectively. Then, we identified the effect of Smoc2 on cell proliferation and cell cycle using CCK-8 and flow cytometry, respectively. The common cell growth signaling influenced by Smoc2 was detected by western blot assay. RESULTS The expression of Smoc2 was significantly higher in HCC tissues compared with CNL tissues. Overexpression of Smoc2 promoted HCC cell proliferation and cell cycle progression. Down-regulation of Smoc2 led to inhibition of cell proliferation and cell cycle progression. Smoc2 had positive effect on ERK and AKT signaling.CONCLUSION Smoc2 promotes the proliferation of HCC cells through accelerating cell cycle progression and might act as an anti-cancer therapeutic target in the future.