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影响肝移植后纤维化发生的宿主及免疫抑制相关因素。

Host and immunosuppression-related factors influencing fibrosis occurrence post liver transplantation.

作者信息

Iacob Speranta, Iacob Razvan, Manea Ioana, Uta Mihaela, Chiosa Andrei, Dumbrava Mona, Becheanu Gabriel, Stoica Luminita, Popa Codruta, Brasoveanu Vlad, Hrehoret Doina, Gheorghe Cristian, Gheorghe Liana, Dima Simona, Popescu Irinel

机构信息

Gastroenterology Department, University of Medicine and Pharmacy "Carol Davila", Bucharest, Romania.

Center for Excellence in Translational Medicine, Bucharest, Romania.

出版信息

Front Pharmacol. 2022 Oct 18;13:1042664. doi: 10.3389/fphar.2022.1042664. eCollection 2022.

DOI:10.3389/fphar.2022.1042664
PMID:36330082
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC9622773/
Abstract

Post liver transplantation (LT) fibrosis has a negative impact on graft function. Cytokine production in the host immune response after LT may contribute to the variable CYP3A-dependent immunosuppressive drug disposition, with subsequent impact on liver fibrogenesis, together with host-related factors. We aimed to investigate whether the cytochrome P4503A53 (CYP3A53) or TBX21 genotypes impact post-LT liver fibrogenesis. Furthermore, the impact of immunosuppressants on cellular apoptosis has been evaluated using human hepatocytes harvested from cirrhotic explanted livers. We have enrolled 98 LT recipients that were followed for occurrence of liver fibrosis for at least 12 months. There was a statistically significant higher trough level of TAC in patients with homozygous CC-TBX21 genotype (7.83 ± 2.84 ng/ml) vs. 5.66 ± 2.16 ng/ml in patients without this genotype ( = 0.009). The following variables were identified as risk factors for fibrosis ≥2: donor age ( = 0.02), neutrophil to lymphocyte ratio ( = 0.04) and TBX21 genotype CC ( = 0.009). In the cell culture model cytometry analysis has indicated the lowest apoptotic cells percentage in human cirrhotic hepatocytes cultures treated with mycophenolate mofetil (MMF) (5%) and TAC + MMF (2%) whereas the highest apoptosis percentage was registered for the TAC alone (11%). The gene expression results are concordant to cytometry study results, indicating the lowest apoptotic effect for MMF and MMF + TAC immunosuppressive regimens. The allele 1993C of the SNP rs4794067 may predispose to the development of late significant fibrosis of the liver graft. MMF-based regimens have a favourable anti-apoptotic profile , supporting its use in case of LT recipients at high risk for liver graft fibrosis.

摘要

肝移植(LT)后纤维化对移植物功能有负面影响。LT后宿主免疫反应中的细胞因子产生可能导致CYP3A依赖的免疫抑制药物处置存在差异,进而影响肝纤维化,同时还受到宿主相关因素的影响。我们旨在研究细胞色素P4503A53(CYP3A53)或TBX21基因型是否会影响LT后肝纤维化的发生。此外,还使用从肝硬化切除肝脏中获取的人肝细胞评估了免疫抑制剂对细胞凋亡的影响。我们招募了98名LT受者,对其肝纤维化的发生情况进行了至少12个月的随访。纯合子CC - TBX21基因型患者的他克莫司(TAC)谷浓度在统计学上显著高于无该基因型患者(7.83±2.84 ng/ml vs. 5.66±2.16 ng/ml,P = 0.009)。以下变量被确定为纤维化≥2的危险因素:供体年龄(P = 0.02)、中性粒细胞与淋巴细胞比值(P = 0.04)和TBX21基因型CC(P = 0.009)。在细胞培养模型中,流式细胞术分析表明,用霉酚酸酯(MMF)(5%)和TAC + MMF(2%)处理的人肝硬化肝细胞培养物中凋亡细胞百分比最低,而单独使用TAC时凋亡百分比最高(11%)。基因表达结果与流式细胞术研究结果一致,表明MMF和MMF + TAC免疫抑制方案的凋亡作用最低。单核苷酸多态性rs4794067的1993C等位基因可能易导致肝移植后期出现明显纤维化。基于MMF的方案具有良好的抗凋亡特性,支持将其用于肝移植受者中肝移植纤维化高危患者。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/74fc/9622773/750a25e1e084/fphar-13-1042664-g002.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/74fc/9622773/598956066aad/fphar-13-1042664-g001.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/74fc/9622773/750a25e1e084/fphar-13-1042664-g002.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/74fc/9622773/598956066aad/fphar-13-1042664-g001.jpg
https://cdn.ncbi.nlm.nih.gov/pmc/blobs/74fc/9622773/750a25e1e084/fphar-13-1042664-g002.jpg

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本文引用的文献

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Heterogeneity and Function of Kupffer Cells in Liver Injury.肝损伤中库普弗细胞的异质性和功能。
Front Immunol. 2022 Jun 27;13:940867. doi: 10.3389/fimmu.2022.940867. eCollection 2022.
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Int J Mol Sci. 2020 Dec 18;21(24):9682. doi: 10.3390/ijms21249682.
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The influence of exposure to immunosuppressive treatment during pregnancy on renal function and rate of apoptosis in native kidneys of female Wistar rats.孕期暴露于免疫抑制治疗对雌性Wistar大鼠天然肾脏的肾功能及细胞凋亡率的影响。
Apoptosis. 2016 Nov;21(11):1240-1248. doi: 10.1007/s10495-016-1281-y.
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