| A Highly Sensitive Anion Exchange Chromatography Method for Measuring cGAS Activity in vitro
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Author:
Date:
2018-10-20
[Abstract] Cyclic GMP-AMP synthase (cGAS) is a pattern recognition receptor (PRR) that senses double stranded DNA (dsDNA) in the cytosol and this leads to the activation of stimulator of interferon genes (STING) via the secondary messenger 2’3’-cyclic GMP-AMP (2’3’-cGAMP). STING then recruits TANK binding kinase 1 (TBK-1) and this complex can phosphorylate and activate interferon regulatory factor 3 (IRF3) leading to the induction of type I interferons and other antiviral genes. The cGAS:DNA complex catalyzes the synthesis of 2’3’-cGAMP and the purpose of the protocol presented here is to measure the in vitro activity of purified cGAS in the presence of dsDNA. The protocol was developed to elucidate the relationship between dsDNA length and the level of cGAS activity. The method involves an in ...
[摘要] 环状GMP-AMP合酶(cGAS)是一种模式识别受体(PRR),可以感知胞质溶胶中的双链DNA(dsDNA),并通过第二信使2'3'来激活干扰素基因刺激物(STING)。环GMP-AMP(2'3'-cGAMP)。然后STING募集TANK结合激酶1(TBK-1),该复合物可磷酸化并激活干扰素调节因子3(IRF3),导致I型干扰素和其他抗病毒基因的诱导。 cGAS:DNA复合物催化2'3'-cGAMP的合成,这里提出的方案的目的是测量在dsDNA存在下纯化的cGAS的体外>活性。开发该方案是为了阐明dsDNA长度与cGAS活性水平之间的关系。该方法涉及与低浓度cGAS和dsDNA的体外>反应,然后使用阴离子交换色谱法定量反应产物。当比较不同DNA片段激活cGAS的能力时,低浓度的cGAS和dsDNA以及该测定的高灵敏度是关键优势。
【背景】细胞胞质内存在双链DNA是DNA或逆转录病毒感染的潜在迹象。核苷酸转移酶cGAS作为感知细胞溶质dsDNA的模式识别受体起作用。 cGAS被dsDNA变构激活并催化ATP和GTP转化为环状二核苷酸2'3'-cGAMP(或简称cGAMP)(Ablasser et al。>,2013; Civril et al 。>,2013; Diner et al。>,2013; Gao et al。>,2013; ...
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| Construction and Cloning of Minigenes for in vivo Analysis of Potential Splice Mutations
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Author:
Date:
2018-03-05
[Abstract] Disease-associated mutations influencing mRNA splicing are referred to as splice mutations. The majority of splice mutations are found on exon-intron boundaries defining canonical donor and acceptor splice sites. However, mutations in the coding region (exonic mutations) can also affect mRNA splicing. Exact knowledge of the disease mechanism of splice mutations is essential for developing optimal treatment strategies. Given the large number of disease-associated mutations thus far identified, there is an unmet need for methods to systematically analyze the effects of pathogenic mutations on mRNA splicing. As splicing can vary between cell types, splice mutations need to be tested under native conditions if possible. A commonly used tool for the analysis of mRNA splicing is the ...
[摘要] 影响mRNA剪接的疾病相关突变称为剪接突变。大多数剪接突变位于确定典型供体和受体剪接位点的外显子 - 内含子边界上。然而,编码区中的突变(外显子突变)也可影响mRNA剪接。准确了解剪接突变的疾病机制对于开发最佳治疗策略至关重要。鉴于迄今为止鉴定的大量疾病相关突变,尚未满足对系统分析致病突变对mRNA剪接的影响的方法的需求。由于不同细胞类型之间的拼接可能不同,如果可能的话,拼接突变需要在天然条件下进行测试。一种常用的分析mRNA剪接的工具是携带外显子和内含子序列的小基因的构建。在这里,我们描述了设计和克隆到重组腺相关病毒(rAAV)载体中用于基因递送和在本地环境中调查mRNA剪接的方案。该协议是为了基于小基因的视网膜细胞中mRNA剪接分析而开发的,但是原则上它适用于任何可以用rAAV载体转导的细胞类型。
【背景】预计大部分疾病相关突变(至少15%)会导致异常的mRNA剪接(Cartegni等,2002; Singh和Cooper,2012; Sterne-Weiler和Sanford,2014年)。 '经典'剪接突变是影响定义5'和3'剪接位点(分别为供体和受体剪接位点)的规范序列的突变。然而,剪接突变也可能发生在其他非编码区和编码区(Wang和Cooper,2007; ...
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| Single-step Marker Switching in Schizosaccharomyces pombe Using a Lithium Acetate Transformation Protocol
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Author:
Date:
2016-12-20
[Abstract] The ability to utilize different selectable markers for tagging or mutating multiple genes in Schizosaccharomyces pombe is hampered by the historical use of only two selectable markers, ura4+ and kanMX6; the latter conferring resistance to the antibiotic G418 (geneticin). More markers have been described recently, but introducing these into yeast cells often requires strain construction from scratch. To overcome this problem we and other groups have created transformation cassettes with flanking homologies to ura4+ and kanMX6 which enable an efficient and time-saving way to exchange markers in existing mutated or tagged fission yeast strains.
Here, we present a protocol for single-step marker switching by ...
[摘要] 利用不同的选择标记来标记或突变粟酒裂殖酵母中的多个基因的能力受到仅仅两种可选择标记的历史使用的阻碍,即 +和 kanMX6 ;后者赋予抗生素G418(遗传霉素)抗性。最近已经描述了更多的标记物,但是将它们引入酵母细胞通常需要从头开始施加应变。为了克服这个问题,我们和其他团队已经创建了具有与 + 和 kanMX6 的侧翼同源性的转换盒,这使得能够有效和省时的方式在现有的突变或标记的裂变酵母菌株中交换标记。
 在这里,我们提出了裂殖酵母,粟酒裂殖酵母(Schizosaccharomyces pombe)中醋酸锌转化的单步标记转换方案。以下我们将介绍如何将 ura4 + 标记交换到kanMX6 , natMX4 或 hphMX4标记,其分别对抗生素G418,海参(clonNAT)或潮霉素B提供抗性。我们还详细介绍了如何交换营养标记的任何 MX 标记,例如 arg3 + , his3 + , leu1 + 和 ura4 + 。
背景 这种用于粟酒裂殖酵母的单步骤标记交换方案允许将标记有类型的抗生素标记的任何标记或突变的基因替换为营养标记物(含有arg3 + , + ,并且已经构建了 ura4 + )并且为任何 MX交换遗传 ura4 + ...
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