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Biologia

小规模提取 秀丽隐杆线虫 基因组DNA

Published: June 07, 2022
doi:
10.3791/63716
, ,
1Department of Biology,Texas Woman’s University

Summary

这里介绍的是使用市售组织试剂盒从一只或几只动物中直接和相对快速地分离 秀丽隐杆线虫 基因组DNA的描述。所得的gDNA制剂是PCR的合适模板。

Abstract

从单个或几个 秀丽隐杆线虫 中提取基因组DNA具有许多下游应用,包括用于基因分型系,克隆和测序的PCR。传统的基于蛋白酶K的方法从 秀丽隐杆线虫 中提取基因组DNA需要几个小时。有效打开 秀丽隐杆线虫 角质层和提取基因组DNA的商业提取试剂盒是有限的。本文介绍了一种简单,快速(约15分钟)且具有成本效益的提取 秀丽隐杆线虫 基因组DNA的方法,该方法适用于课堂和研究应用。这种DNA提取方法经过优化,使用单个或几个晚幼虫(L4)或成体线虫作为获得可靠模板进行PCR的起始材料。结果表明,DNA质量适用于通过PCR扩增不同大小的基因靶标,即使在每次反应中稀释到单个成虫DNA的五十分之一时,也可以对单个或少数动物进行基因分型。所报告的实验方案可以可靠地用于从单个或一小个 秀丽隐杆线虫 样本中快速生成DNA模板,用于基于PCR的应用。

Introduction

在这里,提出了两种用于秀 丽隐杆线虫 裂解的相关方案,以使DNA可用于基于PCR的应用。PCR是一种常用的分子技术,用于许多应用,包括用于克隆和测序的DNA片段的基因分型和扩增等。小(1毫米),自由生活的蛔虫 秀丽隐杆线虫 是生物学研究的流行动物系统。从单个动物或少数动物中获得合适的基因组DNA足以通过PCR扩增序列。晚期L4幼虫和成虫在 子宫仅含有约1,000个体细胞(包括一些多核多倍体细胞),生殖细胞和(如果动物是妊娠雌雄同体)后代。然而,这些动物受到角质层的保护,必须破坏角质层以提取基因组DNA2。制备用于PCR的线虫基因组DNA模板的标准方法涉及多个步骤,需要几个小时。首先将动物在含有蛋白酶K(−70°C或更低)的蠕虫裂解缓冲液中冷冻至少15-45分钟(某些方案建议更长)3456。这一步打开了动物。

冷冻后,将动物在60-65°C下孵育1小时以使蛋白酶K起作用,然后将酶在95°C下灭活15-30分钟。 蛋白酶K破坏降解DNA的核酸酶。在PCR之前蛋白酶K失活对于防止蛋白酶K降解DNA聚合酶非常重要。这里描述的两种基于试剂盒的方案是从单个动物或几个线虫中提取基因组DNA的快速,可靠且具有成本效益的方法,用于日常研究和教学实验室应用。所使用的试剂盒最初由制造商优化,以从动物组织,唾液和毛发中提取DNA7。它使用专有的组织制备溶液和提取溶液来裂解细胞并使基因组DNA易于访问。然后,专有的中和溶液中和可能抑制PCR的组分(例如,盐,离子和Mg2 +结合分子)。

在基因分型时,可以测试单个动物。在确定菌株是否纯合时,从单个动物中测试六个或更多后代可以高度肯定一个品系是否纯合(从杂合亲本随机挑选六个纯合突变后代的几率为0.02%[(1/4)6 ×100%= 0.02%])。该方法1)简单明了,步骤比蛋白酶K方法少,2)将模板制备时间减少到15分钟。这项工作的结果表明,所开发的方案在从单个或几个蠕虫中提取基因组DNA方面具有强大的作用,这些基因组DNA可以可靠地用于不需要高度纯化的DNA的下游应用,包括PCR。

Protocol

1. 秀丽隐杆线虫的 维持 注意:N2(野生型)和 blmp-1(tm548)C.秀丽隐杆线虫 菌株在20°C下维持在标准线虫生长培养基(NGM)板上。 通过将23.005gNGM粉末溶解在2L烧瓶中的973mL水中来制备NGM板。用铝箔(或允许排气的可高温高压灭菌盖)盖住烧瓶开口,并用高压灭菌胶带固定盖子。高压灭菌器溶解粉末并以至少30分钟的灭菌循环对内容物进行灭菌?…

Representative Results

使用商业试剂盒或传统裂解方案从单个或几个野生型成虫中提取基因组DNA,以比较这两种方法的疗效。然后将这些裂解物用作PCR的模板,以扩增〜2,100 bp的较大靶标(编码 blmp-1)或〜500 bp的较小靶标(编码 sma-10的一部分)。两种方法都成功产生了适当的PCR产物(图1A)。 接下来,证明了试剂盒提取的基因组DNA作为各种DNA聚合酶模板的能力…

Discussion

确定 秀丽隐杆线虫 的基因型是进行遗传杂交以创建新的 秀丽隐杆线虫 菌株的重要步骤。使用单个或几个 秀丽隐杆线虫进行 基因组DNA提取是秀 丽隐杆线虫基因分型的关键步骤。该协议描述了使用商业试剂盒从 秀丽隐杆线虫 中提取基因组DNA。此方法速度快,工作可靠。使用这种方法提取的基因组DNA可用于下游应用,包括基因分型,测序和克隆。所描述的DNA提取?…

Divulgazioni

The authors have nothing to disclose.

Acknowledgements

N2菌株和 大肠杆菌 OP50细菌是从 Caenorhabditis 遗传学中心(CGC)获得的,该中心由NIH研究基础设施计划办公室(P40 OD010440)资助。 blmp-1(tm548) 菌株来自日本国家生物资源项目。作者感谢WormBase。这项工作得到了NIH R01GM097591对T.L.G.的支持,德克萨斯女子大学对T.L.G.的内部资助,以及TWU的学生研究中心对M.F.L.的支持。

Materials

autoclave tape Defend 43237-2
aluminium foil, heavy duty Reynolds Wrap 2182934
calcium chloride Millipore Sigma 102382 (CAS 10035-04-8)
Extract-N-Amp kit (includes Tissue Preparation Solution, Extraction Solution, and Neutralization Solution) Sigma-Aldrich Co. LLC XNAT2-1KT
Isotemp hotplate/stirrer Fisher Scientific 11-100-495H
LB media, Lennox, capsules MP Biomedicals, LLC 3002-131
magnesium sulfate, 97% pure, anhydrous Thermo Scientific AC413485000 (CAS 7487-88-9)
microcentrifuge Labnet International, Inc. PrismR, C2500-R
NEB Q5U Hot Start High-Fidelity DNA polymerase New England Biolabs, Inc. M0515S "Pol E" used in Supplemental Figure S1, a high-speed, high-fidelity polymerase (20–30 s/kb)
NGM media powder US Biological Life Sciences N1000
Phusion High-Fidelity PCR Master Mix with HF Buffer New England Biolabs, Inc. M0531S "Pol D" in Figure 1B, a high-speed, high-fidelity polymerase (15–30 s/kb)
primers Integrated DNA Technologies custom DNA oligos
PrimeSTAR GXL polymerase Takara Bio Inc. R050B "Pol C" in Figure 1B, a high-fidelity polymerase (1 min/kb) for GC-rich templates and templates up to 30 kb
Quick-Load Purple 2-log DNA Ladder (0.1–10.0 kb) New England Biolabs, Inc. N0550S
SapphireAmp Fast PCR Master Mix Takara Bio Inc. RR350A "Pol A" in Figure 1B, polymerase used in Figure 1A, C, D, a high-speed polymerase (10 s/kb) for targets up to 5 kb
Sigma ReadyMix Taq PCR reaction mix Sigma-Aldrich Co. LLC P4600 "Pol B" in Figure 1B, a polymerase (1 min/kb) for targets up to 7 kb
SimpliAmp thermal cycler Applied Biosystems A24812
stir bar Fisher Scientific 14-512-126
vortex mixer Fisher Scientific 2215365
worm pick Genesee Scientific Corporation 59-AWP
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Riferimenti

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Tags

Keywords: Caenorhabditis ElegansGenomic DNA ExtractionSmall-scaleClassroomRicercaPCRLysis ProgramExtraction SolutionNeutralization SolutionL4Adult HermaphroditePlatinum Wire PickCentrifugation
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Citazione di questo articolo
Madhu, B., Lakdawala, M. F., Gumienny, T. L. Small-Scale Extraction of Caenorhabditis elegans Genomic DNA. J. Vis. Exp. (184), e63716, doi:10.3791/63716 (2022).
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