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三种用于人类微生物群研究的DNA提取方法和两种测序技术的比较

Comparison of Three DNA Isolation Methods and Two Sequencing Techniques for the Study of the Human Microbiota.

作者信息

Plaza-Díaz Julio, Fernández Mariana F, García Federico, Chueca Natalia, Fontana Luis, Álvarez-Mercado Ana I

机构信息

Institute of Biosanitary Research (ibs.GRANADA), San Cecilio University Clinical Hospital, 18012 Granada, Spain.

School of Health Sciences, International University of La Rioja, 26001 Logroño, Spain.

出版信息

Life (Basel). 2025 Apr 4;15(4):599. doi: 10.3390/life15040599.

Abstract

Breast cancer is the most commonly diagnosed cancer in women and the second leading cause of female death. Altered interactions between the host and the gut microbiota appear to play an influential role in carcinogenesis. Several studies have shown different signatures of the gut microbiota in patients with breast cancer compared to healthy women. Currently, there is disagreement regarding the different DNA isolation and sequencing methodologies for studies on the human microbiota, given that they can influence the interpretation of the results obtained. The goal of this work was to compare (1) three different DNA extraction strategies to minimize the impact of human DNA, and (2) two sequencing strategies (16S rRNA and shotgun) to identify discrepancies in microbiome results. We made use of breast tissue and fecal samples from both healthy women and breast cancer patients who participated in the MICROMA study (reference NCT03885648). DNA was isolated by means of mechanical lysis, trypsin, or saponin. The amount of eukaryotic DNA isolated using the trypsin and saponin methods was lower compared to the mechanical lysis method (mechanical lysis, 89.11 ± 2.32%; trypsin method, 82.63 ± 1.23%; saponin method, 80.53 ± 4.09%). In samples with a predominance of prokaryotic cells, such as feces, 16S rRNA sequencing was the most advantageous approach. For other tissues, which are expected to have a more complex microbial composition, the need for an in-depth evaluation of the multifactorial interaction between the various components of the microbiota makes shotgun sequencing the most appropriate method. As for the three extraction methods evaluated, when sequencing samples other than stool, the trypsin method is the most convenient. For fecal samples, where contamination by host DNA is low, no prior treatment is necessary.

摘要

乳腺癌是女性中最常被诊断出的癌症,也是女性死亡的第二大主要原因。宿主与肠道微生物群之间改变的相互作用似乎在致癌过程中发挥着重要作用。几项研究表明,与健康女性相比,乳腺癌患者的肠道微生物群具有不同的特征。目前,关于人类微生物群研究的不同DNA分离和测序方法存在分歧,因为它们会影响对所得结果的解释。这项工作的目的是比较:(1)三种不同的DNA提取策略,以尽量减少人类DNA的影响;(2)两种测序策略(16S rRNA和鸟枪法),以识别微生物组结果中的差异。我们利用了参与MICROMA研究(参考编号NCT03885648)的健康女性和乳腺癌患者的乳腺组织及粪便样本。通过机械裂解、胰蛋白酶或皂苷来分离DNA。与机械裂解方法相比,使用胰蛋白酶和皂苷方法分离的真核DNA量较低(机械裂解法为89.11±2.32%;胰蛋白酶法为82.63±1.23%;皂苷法为80.53±4.09%)。在以原核细胞为主的样本(如粪便)中,16S rRNA测序是最有利的方法。对于其他预计微生物组成更复杂的组织,由于需要深入评估微生物群各组分之间的多因素相互作用,鸟枪法测序是最合适的方法。至于所评估的三种提取方法,在对粪便以外的样本进行测序时,胰蛋白酶法最方便。对于宿主DNA污染较低的粪便样本,无需事先处理。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/06ae/12028492/20abd888dec8/life-15-00599-g001.jpg

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