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来自溃疡性人体皮肤活检样本的RNA制剂的质量参数。

Quality parameters for RNA preparations from biopsies of ulcerated human skin.

作者信息

Giraldo-Parra Lina, Ramirez Lady Giovanna, Navas Adriana, Gómez María Adelaida

机构信息

Centro Internacional de Entrenamiento e Investigaciones Médicas-CIDEIM, Cali, Valle del Cauca, 760031, Colombia.

Universidad Icesi, Cali, Valle del Cauca, 760031, Colombia.

出版信息

Wellcome Open Res. 2023 Feb 28;7:249. doi: 10.12688/wellcomeopenres.18052.2. eCollection 2022.

Abstract

Obtaining high quality RNA from skin biopsies is complex due the physical composition and high content of nucleases of this tissue. This becomes particularly challenging when using compromised skin samples with necrotic, inflammed or damaged areas, such as those from patients suffering skin conditions, which affect more than 900 million people annually. We evaluated the impact of the biopsy size and tissue preservation method on the quality and quantity of RNA extracts. Skin lesion biopsies were obtained from patients with cutaneous leishmaniasis (CL). Biopsy specimens of 2 mm (n = 10) and 3 mm (n = 59) were preserved in Allprotect® reagent, and 4 mm biopsies in OCT (n = 54). Quality parameters were evaluated using Nanodrop and Bioanalyzer. The informativeness of the extracted samples for downstream analyses was evaluated using RT-qPCR and RNA-Seq. The success rate, based on quality parameters of RNA extraction from tissue biopsies stored in OCT and 2 mm biopsies stored in Allprotect®, was 56% (30/54) and 30% (3/10), respectively. For 3 mm skin biopsies stored in Allprotect® was 93% (55/59). RNA preparations from 3 mm-Allprotect® biopsies had an average RIN of 7.2 ± 0.7, and their integrity was not impacted by sample storage time (up to 200 days at -20°C). RNA products were appropriate for qRT-PCR and RNA-seq. Based on these results, we propose a standardized method for RNA extraction from disrupted skin samples. This protocol was validated with lesion biopsies from CL patients (n = 30), having a success rate of 100%. Our results indicate that a biopsy size of 3 mm in diameter and preservation in Allprotect® for up to 200 days at -20°C, are best to obtain high quality RNA preparations from ulcerated skin lesion biopsy samples.

摘要

由于皮肤活检组织的物理组成和核酸酶含量高,从皮肤活检样本中获取高质量RNA很复杂。当使用有坏死、炎症或损伤区域的受损皮肤样本时,这一挑战尤为突出,比如那些来自患有皮肤疾病患者的样本,每年有超过9亿人受皮肤疾病影响。我们评估了活检样本大小和组织保存方法对RNA提取物质量和数量的影响。皮肤病变活检样本取自皮肤利什曼病(CL)患者。2毫米(n = 10)和3毫米(n = 59)的活检标本保存在Allprotect®试剂中,4毫米的活检标本保存在OCT中(n = 54)。使用Nanodrop和生物分析仪评估质量参数。使用RT-qPCR和RNA测序评估提取样本用于下游分析的信息量。基于保存在OCT中的组织活检样本以及保存在Allprotect®中的2毫米活检样本的RNA提取质量参数,成功率分别为56%(30/54)和30%(3/10)。对于保存在Allprotect®中的3毫米皮肤活检样本,成功率为93%(55/59)。来自3毫米-Allprotect®活检样本的RNA制剂平均RIN为7.2±0.7,其完整性不受样本保存时间(在-20°C下长达200天)的影响。RNA产物适用于qRT-PCR和RNA测序。基于这些结果,我们提出了一种从受损皮肤样本中提取RNA的标准化方法。该方案在CL患者的病变活检样本(n = 30)中得到验证,成功率为100%。我们的结果表明,直径3毫米的活检样本并在-20°C下在Allprotect®中保存长达200天,最有利于从溃疡皮肤病变活检样本中获得高质量的RNA制剂。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/99ac/9984860/2663f662ce99/wellcomeopenres-7-21193-g0000.jpg

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