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Biyokimya

即用型qPCR,用于检测 克氏锥虫 或其他致病微生物的DNA

Published: January 20, 2022
doi:
10.3791/63316
, , ,
1Laboratório de Ciências e Tecnologias Aplicadas em Saúde (LaCTAS), Instituto Carlos Chagas (ICC),Fundação Oswaldo Cruz (Fiocruz), 2Pós-graduação em Engenharia de Bioprocessos e Biotecnologia,Universidade Federal do Paraná (UFPR), 3Pós-graduação em Biociências e Biotecnologia, Instituto Carlos Chagas (ICC),Fundação Oswaldo Cruz (Fiocruz)

Özet

本工作描述了生产用于 克氏锥虫 DNA检测的即用型qPCR的步骤,该qPCR可以预先加载到反应容器中并在冰箱中储存数月。

Abstract

实时荧光定量PCR(qPCR)是一种非常灵敏和精确的技术,可以从大量样品中扩增微量的核酸靶标。它已广泛应用于许多研究领域,并在转基因作物的人体诊断和性状选择等领域实现工业应用。然而,qPCR不是一种防错技术。将所有试剂混合到单个预混液中,随后分配到常规qPCR板的96个孔中可能会导致操作人员错误,例如试剂混合不正确或分配到孔中不准确。这里介绍了一种称为凝胶化的技术,其中预混液中存在的大部分水被试剂取代,这些试剂在提交真空时形成溶胶-凝胶混合物。结果,qPCR试剂在室温下有效保存数周或在2-8 °C下保存数月.此处显示了制备每种溶液的详细信息以及旨在检测克氏锥虫 卫星DNA(satDNA)的凝胶化反应的预期方面。类似的程序可以应用于检测其他生物。开始凝胶化qPCR运行就像从冰箱中取出板,将样品添加到各自的孔中并开始运行一样简单,从而将全板反应的设置时间减少到加载样品所需的时间。此外,可以批量生产和控制凝胶化PCR反应的质量,从而节省时间并避免在运行常规PCR反应时出现常见的操作错误。

Introduction

恰加斯病是在20世纪初在 巴西农村地区发现的,那里的贫困普遍存在12。即使在今天,这种疾病仍然与美洲健康的社会和经济决定因素有关。恰加斯病是双相的,包括急性期和慢性期。它是由 克氏锥 虫寄生虫感染、通过昆虫媒介传播、通过先天途径输血或口服摄入受污染的食物引起的34

恰加斯病的诊断可以通过观察临床症状(尤其是罗马尼亚征)、血涂片显微镜检查、血清学和分子检测(如实时荧光定量 PCR (qPCR) 或等温扩增456789)进行。临床症状和血涂片显微镜检查用于疑似急性感染病例,而寻找抗体则用作无症状患者的筛查工具。由于其敏感性和特异性,qPCR 已被建议用作慢性患者的监测工具、正在接受治疗的急性患者测量血液中寄生虫负荷以及作为治疗失败的替代标志物68,101112.尽管qPCR比目前可用的测试更具敏感性和特异性,但由于运输和储存需要冷冻温度,qPCR在全球贫困地区被有效地阻止了诊断工具131415

为了绕过这一障碍,已经探索了冻干和凝胶化等保护技术1617。虽然冻干可提供多年的保存,但它需要不含甘油的特殊试剂,甘油通常用于酶稳定/保存18。虽然凝胶化已被证明可以提供数月的保存,但它允许使用常规试剂19。凝胶化溶液包括四种组分,每种组分在过程中都有特定的作用:糖海藻糖和黑糖糖在干燥过程中通过还原溶液中的游离水分子来保护生物分子,糖原产生更广泛的保护基质,氨基酸赖氨酸用作自由基清除剂以抑制生物分子羧基之间的氧化反应, 氨基和磷酸基团。这些组分定义了溶胶-凝胶混合物,可防止在干燥过程中损失三级或四级结构,从而有助于维持生物分子在补水时的活性19。一旦在反应管内稳定,反应可以在2-8°C下储存几个月或在21-23°C下储存数周,而不是常规的-20°C。 这种方法已被纳入旨在帮助诊断恰加斯病、疟疾、利什曼病、结核病和环孢子虫病等疾病的测试中13141520

本工作描述了为凝胶化程序准备所需解决方案的所有步骤、过程中的陷阱以及八管条带内即用型凝胶化qPCR的预期最终方面。相同的方案可以适用于单管或96孔板。最后, 克氏锥虫 DNA的检测将显示为对照运行。

Protocol

1. 储备溶液和凝胶化混合物的制备 注意:将制备四种储备溶液(400 mg / mL的melezitose,400 mg / mL的海藻糖,0.75 mg / mL的赖氨酸和200 mg / mL的糖原)并根据 表1 所示的比例混合以产生凝胶化混合物。尽管该方案描述了 10 mL 储备溶液的生产,但它可以适用于较低或较高体积。 美来糖溶液称取 4 g 蜜蜂托糖放入 15 mL 塑料管中,加入 6 mL 无核酸酶?…

Representative Results

形成凝胶化混合物的三种试剂在剧烈涡旋下很容易溶解。然而,糖原需要仔细涡旋以确保粉末完全溶解。不幸的是,剧烈涡旋会产生大量气泡,这使得难以确定溶液的实际体积(图1A-B)。因此,必须让糖原溶液在冰箱中休息,直到气泡中捕获的大部分溶液向下移动到主溶液体。考虑到生产方案和实验室常规,将凝胶板在冰箱中保存过夜(或约8-12小?…

Discussion

近年来,人们强调需要找到更敏感和更具体的技术来帮助诊断热带和被忽视的疾病。虽然寄生虫学(光学显微镜)和血清学检测对流行病学控制很重要,但局限性,特别是在敏感性和床旁适用性方面。DNA扩增技术,如PCR,等温扩增和相应的变异,长期以来一直在实验室环境中使用,但技术障碍使其无法在现场环境中使用。主要障碍之一是试剂的运输和储存需要-20°C的温度。为了补救这种情况,已?…

Açıklamalar

The authors have nothing to disclose.

Acknowledgements

作者感谢Aline Burda Farias为真空烘箱提供的技术援助,并感谢巴拉那分子生物学研究所(IBMP,巴西库里提巴)的行政部门允许使用上述设备。这项工作的部分资金来自 CNPq 445954/2020-5 赠款。

Materials

Bentonite clay bags (activated) Embamat Global Packaging Solutions (Barcelona, Spain) 026157/STD Not to be confused with silica gel packs
Glycogen Amersham Bioscience Cat# US16445
Lysine Acros Organic Cat# 365650250
Melezitoze Sigma-Aldrich Cat# 63620
Nuclease-free water preferred vendor
Oligonucleotides preferred vendor
PCR mastermix preferred vendor or Instituto de Biologia Molecular do Paraná (IBMP, Curitiba, Brazil) Chagas NAT kit
PCR thermocycler preferred vendor
software for vacuum oven Memmert Gmbh Celsius v10.0
Trehalose Sigma-Aldrich Cat# T9531
Trypanosoma cruzi DNA from in-house cultivated parasites, or purchased from accredited vendors such as ATCC
Vacuum oven Memmert Gmbh VO-400
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Referanslar

  1. Lewinsohn, R. Carlos Chagas (1879-1934): the discovery of Trypanosoma cruzi and of American trypanosomiasis (foot-notes to the history of Chagas’s disease). Transactions of the Royal Society of Tropical Medicine and Hygiene. 73 (5), 513-523 (1979).
  2. Bern, C., et al. Evaluation and treatment of Chagas disease in the United States: A systematic review. The Journal of American Medical Association. 298 (18), 2171-2181 (2007).
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  4. Tanowitz, H. B., et al. Chagas’ disease. Clinical Microbiology Reviews. 5 (4), 400-419 (1992).
  5. Rassi, A., Marin-Neto, J. A. Chagas disease. Lancet. 375 (9723), 1388-1402 (2010).
  6. Ramírez, J. C., et al. Analytical validation of quantitative real-time PCR methods for quantification of trypanosoma cruzi DNA in blood samples from chagas disease patients. The Journal of Molecular Diagnostics. 17 (5), 605-615 (2015).
  7. Rivero, R., et al. Rapid detection of Trypanosoma cruzi by colorimetric loop-mediated isothermal amplification (LAMP): A potential novel tool for the detection of congenital Chagas infection. Diagnostic Microbiology and Infectious Disease. 89 (1), 26-28 (2017).
  8. Schijman, A. G. Molecular diagnosis of Trypanosoma cruzi. Acta Tropica. 184, 59-66 (2018).
  9. Besuschio, S. A., et al. Trypanosoma cruzi loop-mediated isothermal amplification (Trypanosoma cruzi Loopamp) kit for detection of congenital, acute and Chagas disease reactivation. Plos Neglected Tropical Diseases. 14 (8), 0008402 (2020).
  10. Duffy, T., et al. Accurate real-time PCR strategy for monitoring bloodstream parasitic loads in chagas disease patients. Plos Neglected Tropical Diseases. 3 (4), (2009).
  11. Melo, M. F., et al. Usefulness of real time PCR to quantify parasite load in serum samples from chronic Chagas disease patients. Parasites & Vectors. 8 (1), 154 (2015).
  12. Parrado, R., et al. Usefulness of serial blood sampling and PCR replicates for treatment monitoring of patients with chronic Chagas disease. Antimicrobial Agents and Chemotherapy. 63 (2), 01191 (2019).
  13. de Rampazzo, R. C. P., et al. A ready-to-use duplex qPCR to detect Leishmania infantum DNA in naturally infected dogs. Veterinary Parasitology. 246, 100-107 (2017).
  14. Rampazzo, R. C. P., et al. Proof of concept for a portable platform for molecular diagnosis of tropical diseases. The Journal of Molecular Diagnostics. 21 (5), 839-851 (2019).
  15. Costa, A. D. T., et al. Ready-to-use qPCR for detection of Cyclospora cayetanensis or Trypanosoma cruzi in food matrices. Food and Waterborne Parasitology. 22, 00111 (2021).
  16. Sun, Y., et al. Pre-storage of gelified reagents in a lab-on-a-foil system for rapid nucleic acid analysis. Lab on a Chip. 13, 1509-1514 (2013).
  17. Kamau, E., et al. Sample-ready multiplex qPCR assay for detection of malaria. Malaria Journal. 13, 158 (2014).
  18. Kasper, J. C., Winter, G., Friess, W. Recent advances and further challenges in lyophilization. European Journal of Pharmaceutics and Biopharmaceutics. 85 (2), 162-169 (2013).
  19. Rosado, P. M. F. S., López, G. L., Seiz, A. M., Alberdi, M. M. Method for preparing stabilised reaction mixtures, which are totally or partially dried, comprising at least one enzyme, reaction mixtures and kits containing said mixtures. PubChem. , (2002).
  20. Ali, N., Bello, G. L., Rossetti, M. L. R., Krieger, M. A., Costa, A. D. T. Demonstration of a fast and easy sample-to-answer protocol for tuberculosis screening in point-of-care settings: A proof of concept study. PLoS One. 15 (12), 0242408 (2020).
  21. Murphy, H. R., Lee, S., da Silva, A. J. Evaluation of an improved U.S. food and drug administration method for the detection of Cyclospora cayetanensis in produce using real-time PCR. Journal of Food Protection. 80 (7), 1133-1144 (2017).
  22. Iglesias, N., et al. Performance of a new gelled nested PCR test for the diagnosis of imported malaria: comparison with microscopy, rapid diagnostic test, and real-time PCR. Parasitology Research. 113 (7), 2587-2591 (2014).
  23. Alonso-Padilla, J., Gallego, M., Schijman, A. G., Gascon, J. Molecular diagnostics for Chagas disease: up to date and novel methodologies. Expert Review of Molecular Diagnostics. 17 (7), 699-710 (2017).

Etiketler

QPCRTrypanosoma CruziPathogenic OrganismsGelification ProtocolReady-to-use QPCRQuality ControlMelezitoseTrehaloseGlycogenLysineStock Solutions

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Costa, A. D. T., Amadei, S. S., Bertão-Santos, A., Rodrigues, T. Ready-To-Use qPCR for Detection of DNA from Trypanosoma cruzi or Other Pathogenic Organisms. J. Vis. Exp. (179), e63316, doi:10.3791/63316 (2022).
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