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相关概念视频

Next-generation Sequencing03:00

Next-generation Sequencing

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The first human genome sequencing project cost $2.7 billion and was declared complete in 2003, after 15 years of international cooperation and collaboration between several research teams and funding agencies. Today, with the advent of next-generation sequencing technologies, the cost and time of sequencing a human genome have dropped over 100 fold.
Next-Generation Sequencing Methods
Although all next-generation methods use different technologies, they all share a set of standard features....
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相关实验视频

Updated: Jun 6, 2025

DNAzyme-dependent Analysis of rRNA 2&#8217;-O-Methylation
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DNAzyme-dependent Analysis of rRNA 2’-O-Methylation

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产生snoRNA引导的可编程2'-O-甲基化.

Justin Zhao, Eric Cockman, Xinhe Yin

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    此摘要是机器生成的。

    这项研究引入了一种新的测定方法,以验证对RNA功能至关重要的2'-O-甲基化 (Nm) 位点. 合成的小核子RNAs (snoRNAs) 可以引导这些修改,影响基因表达和翻译效率.

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    科学领域:

    • 分子生物学分子生物学
    • 在RNA生物学,RNA生物学.
    • 表观遗传学 在表观遗传学中,表观遗传学是指表观遗传学.

    背景情况:

    • 小核RNAs (snoRNAs) 指导2 -O-甲基化 (Nm) 修改,这是RNA处理所必需的.
    • 目前用于绘制Nm位点的方法,特别是信使RNA (mRNA) 的方法,缺乏验证和共识.
    • 需要一种经过验证的技术来推进Nm修饰及其在基因表达中的作用的研究.

    研究的目的:

    • 在单核酸分辨率下开发和验证一种用于量化2 -O-甲基化 (Nm) 的新型试验.
    • 研究合成snoRNAs在指导Nm修改中的潜力.
    • 探索Nm修改对基因表达的影响,包括mRNA丰度和翻译效率.

    主要方法:

    • 开发和应用基于RNase H的Nm-VAQ试验,用于跨RNA物种的Nm量化.
    • 优化对像mRNAs这样的低丰度转录的测试.
    • 合成snoRNAs的设计和利用,以指导Nm修饰在遗传淘汰模型和记者分析中.

    主要成果:

    • 该Nm-VAQ试验成功量化了单核酸分辨率在rRNA,snRNA和mRNA中的Nm修饰.
    • 优化的试验使得在低丰度转录中研究Nm成为可能.
    • 合成的snoRNAs可以被设计为指导Nm到特定的位置,在淘汰模式中进行救援修改,并影响记者基因表达 (luciferase).

    结论:

    • 基于RNase H的Nm-VAQ试验为Nm映射提供了一个关键的验证工具.
    • 合成的snoRNA为研究和操纵Nm修改提供了一个强大的平台.
    • 由snoRNAs引导的Nm修改通过影响mRNA丰度和翻译效率,显著影响基因表达.