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从保存在稳定溶液中的髂骨活检组织中分离矿化骨和骨髓mRNA:一项比较研究。

Isolating mineralized bone and bone marrow mRNA from transiliac bone biopsies stored in a stabilizing solution: A comparative study.

作者信息

de Loor Henriette, Smout Dieter, Jørgensen Hanne, Meng Catarina, Van Craenenbroeck Amaryllis H, Evenepoel Pieter

机构信息

Department of Microbiology, Immunology and Transplantation, Nephrology and Renal Transplantation Research Group, KU Leuven, Leuven, Belgium.

Department of Kidney Diseases, Aarhus University Hospital, Aarhus, Denmark.

出版信息

Bone Rep. 2022 Sep 28;17:101624. doi: 10.1016/j.bonr.2022.101624. eCollection 2022 Dec.

Abstract

The molecular mechanisms underlying metabolic bone diseases, including renal osteodystrophy, are poorly understood. Transcriptomics are increasingly used to characterize biological molecular networks and prove promising in identifying therapeutic targets and biomarkers. A reliable method for obtaining sufficient amounts of high quality RNA from human bone biopsies is a prerequisite for the implementation of molecular diagnostics in clinical research and practice. The present study aimed to develop a simple and adequate method for isolating bone and bone marrow mRNA from transiliac bone biopsies. Several storage, separation, and extraction procedures were compared. The procedure was optimized in pig samples and subsequently validated in human samples. Appropriate amounts of mineralized bone and bone marrow mRNA of moderate to high quality were obtained from transiliac bone biopsies that were immersed in the stabilizing solution Allprotect Tissue Reagent at room temperature for up to 3 days prior to freezing. After thawing, bone marrow and mineralized bone were separated by a multistep centrifugation procedure and subsequently disrupted and homogenized by a bead crusher. Appropriate separation of mineralized bone and bone marrow was confirmed by discriminatory gene expression profiles.

摘要

包括肾性骨营养不良在内的代谢性骨病的分子机制尚不清楚。转录组学越来越多地用于表征生物分子网络,并在识别治疗靶点和生物标志物方面显示出前景。从人类骨活检中获得足够数量高质量RNA的可靠方法是在临床研究和实践中实施分子诊断的前提条件。本研究旨在开发一种从髂骨活检中分离骨和骨髓mRNA的简单且合适的方法。比较了几种储存、分离和提取程序。该程序在猪样本中进行了优化,随后在人类样本中进行了验证。从在冷冻前于室温下在稳定溶液Allprotect Tissue Reagent中浸泡长达3天的髂骨活检中,获得了适量的中等至高质量的矿化骨和骨髓mRNA。解冻后,通过多步离心程序分离骨髓和矿化骨,随后用珠磨仪破碎并匀浆。通过差异基因表达谱证实了矿化骨和骨髓的适当分离。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/e152/9551114/08954b929cad/ga1.jpg

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