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S100钙结合蛋白A6及相关长链非编码核糖核酸作为原发性胆汁性胆管炎诊断和分期的生物标志物

S100 calcium binding protein A6 and associated long noncoding ribonucleic acids as biomarkers in the diagnosis and staging of primary biliary cholangitis.

作者信息

Dong Xi-Hua, Dai Di, Yang Zhi-Dong, Yu Xiao-Ou, Li Hua, Kang Hui

机构信息

Department of Laboratory Medicine, The First Affiliated Hospital of China Medical University, Shenyang 110001, Liaoning Province, China.

出版信息

World J Gastroenterol. 2021 May 7;27(17):1973-1992. doi: 10.3748/wjg.v27.i17.1973.

DOI:10.3748/wjg.v27.i17.1973
PMID:34007134
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC8108032/
Abstract

BACKGROUND

Primary biliary cholangitis (PBC) is a chronic and slowly progressing cholestatic disease, which causes damage to the small intrahepatic bile duct by immuno-regulation, and may lead to cholestasis, liver fibrosis, cirrhosis and, eventually, liver failure.

AIM

To explore the potential diagnosis and staging value of plasma S100 calcium binding protein A6 (S100A6) messenger ribonucleic acid (mRNA), LINC00312, LINC00472, and LINC01257 in primary biliary cholangitis.

METHODS

A total of 145 PBC patients and 110 healthy controls (HCs) were enrolled. Among them, 80 PBC patients and 60 HCs were used as the training set, and 65 PBC patients and 50 HCs were used as the validation set. The relative expression levels of plasma S100A6 mRNA, long noncoding ribonucleic acids LINC00312, LINC00472 and LINC01257 were analyzed using quantitative reverse transcription-polymerase chain reaction. The bile duct ligation (BDL) mouse model was used to simulate PBC. Then double immunofluorescence was conducted to verify the overexpression of S100A6 protein in intrahepatic bile duct cells of BDL mice. Human intrahepatic biliary epithelial cells were treated with glycochenodeoxycholate to simulate the cholestatic environment of intrahepatic biliary epithelial cells in PBC.

RESULTS

The expression of S100A6 protein in intrahepatic bile duct cells was up-regulated in the BDL mouse model compared with sham mice. The relative expression levels of plasma S100A6 mRNA, log10 LINC00472 and LINC01257 were up-regulated while LINC00312 was down-regulated in plasma of PBC patients compared with HCs (3.01 ± 1.04 2.09 ± 0.87, < 0.0001; 2.46 ± 1.03 1.77 ± 0.84, < 0.0001; 3.49 ± 1.64 2.37 ± 0.96, < 0.0001; 1.70 ± 0.33 2.07 ± 0.53, < 0.0001, respectively). The relative expression levels of S100A6 mRNA, LINC00472 and LINC01257 were up-regulated and LINC00312 was down-regulated in human intrahepatic biliary epithelial cells treated with glycochenodeoxycholate compared with control (2.97 ± 0.43 1.09 ± 0.08, = 0.0018; 2.70 ± 0.26 1.10 ± 0.10, = 0.0006; 2.23 ± 0.21 1.10 ± 0.10, = 0.0011; 1.20 ± 0.04 3.03 ± 0.15, < 0.0001, respectively). The mean expression of S100A6 in the advanced stage (III and IV) of PBC was up-regulated compared to that in HCs and the early stage (II) (3.38 ± 0.71 2.09 ± 0.87, < 0.0001; 3.38 ± 0.71 2.57 ± 1.21, = 0.0003, respectively); and in the early stage (II), it was higher than that in HCs (2.57 ± 1.21 2.09 ± 0.87, = 0.03). The mean expression of LINC00312 in the advanced stage was lower than that in the early stage and HCs (1.39 ± 0.29 1.56 ± 0.33, = 0.01; 1.39 ± 0.29 2.07 ± 0.53, < 0.0001, respectively); in addition, the mean expression of LINC00312 in the early stage was lower than that in HCs (1.56 ± 0.33 2.07 ± 0.53, < 0.0001). The mean expression of log10 LINC00472 in the advanced stage was higher than those in the early stage and HCs (2.99 ± 0.87 1.81 ± 0.83, < 0.0001; 2.99 ± 0.87 1.77 ± 0.84, < 0.0001, respectively). The mean expression of LINC01257 in both the early stage and advanced stage were up-regulated compared with HCs (3.88 ± 1.55 2.37 ± 0.96, < 0.0001; 3.57 ± 1.79 2.37 ± 0.96, < 0.0001, respectively). The areas under the curves (AUC) for S100A6, LINC00312, log10 LINC00472 and LINC01257 in PBC diagnosis were 0.759, 0.7292, 0.6942 and 0.7158, respectively. Furthermore, the AUC for these four genes in PBC staging were 0.666, 0.661, 0.839 and 0.5549, respectively. The expression levels of S100A6 mRNA, log10 LINC00472, and LINC01257 in plasma of PBC patients were decreased (2.35 ± 1.02 3.06 ± 1.04, = 0.0018; 1.99 ± 0.83 2.33 ± 0.96, = 0.036; 2.84 ± 0.92 3.69 ± 1.54, = 0.0006), and the expression level of LINC00312 was increased (1.95 ± 0.35 1.73 ± 0.32, = 0.0007) after treatment compared with before treatment using the paired -test. Relative expression of S100A6 mRNA was positively correlated with log10 LINC00472 ( = 0.683, < 0.0001); serum level of collagen type IV was positively correlated with the relative expression of log10 LINC00472 ( = 0.482, < 0.0001); relative expression of S100A6 mRNA was positively correlated with the serum level of collagen type IV ( = 0.732, < 0.0001). The AUC for the four biomarkers obtained in the validation set were close to the training set.

CONCLUSION

These four genes may potentially act as novel biomarkers for the diagnosis of PBC. Moreover, LINC00472 acts as a potential biomarker for staging in PBC.

摘要

背景

原发性胆汁性胆管炎(PBC)是一种慢性、进展缓慢的胆汁淤积性疾病,通过免疫调节对肝内小胆管造成损伤,可能导致胆汁淤积、肝纤维化、肝硬化,最终发展为肝衰竭。

目的

探讨血浆S100钙结合蛋白A6(S100A6)信使核糖核酸(mRNA)、LINC00312、LINC00472和LINC01257在原发性胆汁性胆管炎中的潜在诊断及分期价值。

方法

共纳入145例PBC患者和110例健康对照(HCs)。其中,80例PBC患者和60例HCs作为训练集,65例PBC患者和50例HCs作为验证集。采用定量逆转录-聚合酶链反应分析血浆S100A6 mRNA、长链非编码核糖核酸LINC00312、LINC00472和LINC01257的相对表达水平。采用胆管结扎(BDL)小鼠模型模拟PBC。然后进行双重免疫荧光以验证BDL小鼠肝内胆管细胞中S100A6蛋白的过表达。用人肝内胆管上皮细胞用甘氨鹅脱氧胆酸盐处理以模拟PBC中肝内胆管上皮细胞的胆汁淤积环境。

结果

与假手术小鼠相比,BDL小鼠模型中肝内胆管细胞S100A6蛋白表达上调。与HCs相比,PBC患者血浆中S100A6 mRNA、log10 LINC00472和LINC01257的相对表达水平上调,而LINC00312下调(分别为3.01±1.04对2.09±0.87,P<0.0001;2.46±1.03对1.77±0.84,P<0.0001;3.49±1.64对2.37±0.96,P<0.0001;1.70±0.33对2.07±0.53,P<0.0001)。与对照组相比,用甘氨鹅脱氧胆酸盐处理的人肝内胆管上皮细胞中S100A6 mRNA、LINC00472和LINC01257的相对表达水平上调,而LINC00312下调(分别为2.97±0.43对1.09±0.08,P = 0.0018;2.70±0.26对1.10±0.1, P = 0.0006;2.23±0.21对1.10±0.10,P = 0.0011;1.20±0.04对3.03±0.15,P<0.0001)。PBC晚期(III和IV期)S100A6的平均表达水平高于HCs和早期(II期)(分别为3.38±0.71对2.09±0.87,P<0.0001;3.38±0.71对2.57±1.21,P = 0.0003);在早期(II期),其高于HCs(2.57±1.21对2.09±0.87,P = 0.03)。晚期LINC00312的平均表达水平低于早期和HCs(分别为1.39±0.29对1.56±0.33,P = 0.01;1.39±0.29对2.07±0.53,P<0.0001);此外,早期LINC00312的平均表达水平低于HCs(1.56±0.33对2.07±0.53,P<0.0001)。晚期log10 LINC00472的平均表达水平高于早期和HCs(分别为2.99±0.87对1.81±0.83,P<0.0001;2.99±0.87对1.77±0.84,P<0.0001)。早期和晚期LINC01257的平均表达水平均高于HCs(分别为3.88±1.55对2.37±0.96,P<0.0001;3.57±1.79对2.37±0.96,P<0.0001)。PBC诊断中S100A6、LINC00312、log10 LINC00472和LINC01257的曲线下面积(AUC)分别为0.759、0.7292、0.6942和0.7158。此外,这四个基因在PBC分期中的AUC分别为0.666、0.661、0.839和0.5549。配对t检验显示,与治疗前相比,PBC患者治疗后血浆中S100A6 mRNA、log10 LINC00472和LINC01257的表达水平降低(分别为2.35±1.02对3.06±1.04,P = 0.0018;1.99±0.83对2.33±0.96,P = 0.036;2.84±0.92对3.69±1.54,P = 0.0006),而LINC00312的表达水平升高(1.95±0.35对1.73±0.32,P = 0.0007)。S100A6 mRNA的相对表达与log10 LINC00472呈正相关(r = 0.683,P<0.0001);IV型胶原血清水平与log10 LINC00472的相对表达呈正相关(r = 0.482,P<0.0001);S100A6 mRNA的相对表达与IV型胶原血清水平呈正相关(r = 0.732,P<0.0001)。验证集中获得的四个生物标志物的AUC与训练集接近。

结论

这四个基因可能作为PBC诊断的新型生物标志物。此外,LINC00472作为PBC分期的潜在生物标志物。

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9
Hydrophobic bile acids suppress expression of AE2 in biliary epithelial cells and induce bile duct inflammation in primary biliary cholangitis.疏水性胆汁酸抑制胆汁上皮细胞中 AE2 的表达,并在原发性胆汁性胆管炎中诱导胆管炎症。
J Autoimmun. 2016 Dec;75:150-160. doi: 10.1016/j.jaut.2016.08.006. Epub 2016 Aug 31.
10
Noncoding RNA: Current Deep Sequencing Data Analysis Approaches and Challenges.非编码RNA:当前深度测序数据分析方法与挑战
Hum Mutat. 2016 Dec;37(12):1283-1298. doi: 10.1002/humu.23066. Epub 2016 Sep 5.