Family-specific degenerate primer design: a tool to design consensus degenerated oligonucleotides.

Biotechnology Research International Pub Date : 2013-01-01 Epub Date: 2013-02-21 DOI:10.1155/2013/383646

Javier Alonso Iserte, Betina Ines Stephan, Sandra Elizabeth Goñi, Cristina Silvia Borio, Pablo Daniel Ghiringhelli, Mario Enrique Lozano

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引用次数: 41

Abstract

Designing degenerate PCR primers for templates of unknown nucleotide sequence may be a very difficult task. In this paper, we present a new method to design degenerate primers, implemented in family-specific degenerate primer design (FAS-DPD) computer software, for which the starting point is a multiple alignment of related amino acids or nucleotide sequences. To assess their efficiency, four different genome collections were used, covering a wide range of genomic lengths: Arenavirus (10 × 10(4) nucleotides), Baculovirus (0.9 × 10(5) to 1.8 × 10(5) bp), Lactobacillus sp. (1 × 10(6) to 2 × 10(6) bp), and Pseudomonas sp. (4 × 10(6) to 7 × 10(6) bp). In each case, FAS-DPD designed primers were tested computationally to measure specificity. Designed primers for Arenavirus and Baculovirus were tested experimentally. The method presented here is useful for designing degenerate primers on collections of related protein sequences, allowing detection of new family members.

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家族特异性退化引物设计:一种设计一致退化寡核苷酸的工具。

设计未知核苷酸序列模板的退化PCR引物是一项非常困难的任务。在本文中，我们提出了一种设计退化引物的新方法，该方法在家族特异性退化引物设计(FAS-DPD)计算机软件中实现，其起点是相关氨基酸或核苷酸序列的多重比对。为了评估它们的效率，使用了四种不同的基因组集合，涵盖了广泛的基因组长度:沙粒病毒(10 × 10(4)个核苷酸)、杆状病毒(0.9 × 10(5)至1.8 × 10(5) bp)、乳酸杆菌(1 × 10(6)至2 × 10(6) bp)和假单胞菌(4 × 10(6)至7 × 10(6) bp)。在每种情况下，通过计算测试FAS-DPD设计的引物以测量特异性。设计的引物对沙粒病毒和杆状病毒进行了实验检测。本文提出的方法可用于设计相关蛋白序列集合上的退化引物，从而检测新的家族成员。

本文章由计算机程序翻译，如有差异，请以英文原文为准。

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Biotechnology Research International

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