| RNA Capping by Transcription Initiation with Non-canonical Initiating Nucleotides (NCINs): Determination of Relative Efficiencies of Transcription Initiation with NCINs and NTPs
|
|
Author:
Date:
2017-06-20
[Abstract] It recently has been established that adenine-containing cofactors, including nicotinamide adenine dinucleotide (NAD+), reduced nicotinamide adenine dinucleotide (NADH), and 3’-desphospho-coenzyme A (dpCoA), can serve as ‘non-canonical initiating nucleotides’ (NCINs) for transcription initiation by bacterial and eukaryotic cellular RNA polymerases (RNAPs) and that the efficiency of the reaction is determined by promoter sequence (Bird et al., 2016). Here we describe a protocol to quantify the relative efficiencies of transcription initiation using an NCIN vs. transcription initiation using a nucleoside triphosphate (NTP) for a given promoter sequence.
[摘要] 最近已经确定,含有腺嘌呤的辅因子,包括烟酰胺腺嘌呤二核苷酸(NAD +),还原型烟酰胺腺嘌呤二核苷酸(NADH)和3'-脱磷酸辅酶A(dpCoA)可以作为“非规范起始核苷酸” NCIN),用于通过细菌和真核细胞RNA聚合酶(RNAP)进行转录起始,并且通过启动子序列确定反应的效率(Bird等,2016)。 在这里,我们描述了使用NCIN与使用三磷酸核苷(NTP)对于给定启动子序列的转录起始来定量转录起始的相对效率的方案。
【背景】在细菌,古细菌和真核生物中的转录由序列,结构和机制保守的多亚基RNA聚合酶(RNAPs)进行(Ebright,2000; Lane和Darst,2010)。为了启动转录,RNAP与一个或多个引发因子一起结合称为“启动子”的特异性DNA序列,并解开启动子DNA以形成含有未解链“转录泡”的RNAP启动子开放复合物(RPo)(图1A; Ruff等人,2015)。 RNAP然后通过扩增(“剔除”)或收缩(“抗锯齿”)转录起始点来选择转录起始位点,以将转录起始位点的核苷酸置于RNAP活性中心起始位点(“i位点”)和扩增位点'i + 1位点')结合i位点的互补起始核苷酸底物和“i + 1”位点的互补延伸底物,并催化磷酸二酯键形成产生初始RNA产物(Winkelman等, 2016)。
在标准的从头转录启动中,起始底物是核苷三磷酸(NTP),通常为ATP或GTP(Nickels ...
|
|
|
| CRISPR/Cas9 Editing of the Bacillus subtilis Genome
|
|
Author:
Date:
2017-04-20
[Abstract] A fundamental procedure for most modern biologists is the genetic manipulation of the organism under study. Although many different methods for editing bacterial genomes have been used in laboratories for decades, the adaptation of CRISPR/Cas9 technology to bacterial genetics has allowed researchers to manipulate bacterial genomes with unparalleled facility. CRISPR/Cas9 has allowed for genome edits to be more precise, while also increasing the efficiency of transferring mutations into a variety of genetic backgrounds. As a result, the advantages are realized in tractable organisms and organisms that have been refractory to genetic manipulation. Here, we describe our method for editing the genome of the bacterium Bacillus subtilis. Our method is highly efficient, resulting in ...
[摘要] 大多数现代生物学家的基本过程是研究生物体的遗传操作。尽管许多不同的方法用于编辑细菌基因组已经在实验室中使用了数十年,但CRISPR / Cas9技术对细菌遗传学的适应使得研究人员能够以无与伦比的设施来操纵细菌基因组。 CRISPR / Cas9允许基因组编辑更精确,同时也提高将突变转移到各种遗传背景的效率。因此,在遗传操作难以处理的易处理生物和生物体中实现了这些优点。在这里,我们描述了我们编辑枯草芽孢杆菌细菌基因组的方法。我们的方法是高效的,导致精确,无标记的突变。此外,在产生编辑质粒之后,可以将突变快速导入几个遗传背景,大大增加可进行遗传分析的速度。
枯草芽孢杆菌是高度易处理的革兰氏阳性菌。遗传研究适用于使用多种载体通过同源重组快速有效地引入突变。尽管有许多不同的方法来引入B突变。 subtilis,每种方法都有其局限性。一种简单而简单的方法,用于在B中进行突变。枯草芽孢杆菌是基因破坏,其中将质粒整合到感兴趣的基因内(Vagner等人,1998)。主要的局限性包括:1)扰乱操纵子的极地作用的潜力; 2)引进和保留外来DNA; 3)一旦使用抗生素耐药性盒,如果在其他突变的背景下研究给定的突变,则研究者必须使用不同的盒;和4)该方法限于靶向整个基因,并且不能产生更精确的点突变。 ...
|
|
|
| Measurement of Transferrin- and Non-transferrin-bound Iron Uptake by Mouse Tissues
|
|
Author:
Date:
2016-09-05
[Abstract] Iron in blood plasma is bound to its transport protein transferrin, which delivers iron to most tissues. In iron overload and certain pathological conditions, the carrying capacity of transferrin can become exceeded, giving rise to non-transferrin-bound iron, which is taken up preferentially by the liver, kidney, pancreas, and heart. The measurement of tissue transferrin- and non-transferrin-bound iron (TBI and NTBI, respectively) uptake in vivo can be achieved via intravenous administration of 59Fe-labeled TBI or NTBI followed by gamma counting of various organs. Here we describe a detailed protocol for the measurement of TBI and NTBI uptake by mouse tissues.
[摘要] 血浆中的铁结合其转运蛋白转铁蛋白,其将铁递送至大多数组织。 在铁过载和某些病理状况下,转铁蛋白的携带能力可能超过,导致非转铁蛋白结合的铁,其优先被肝脏,肾脏,胰腺和心脏摄取。 分别测量组织转铁蛋白和非转铁蛋白结合的铁(分别为TBI和NTBI)在体内的摄取可以通过静脉内施用59 Fe标记的TBI或 NTBI,然后是各种器官的γ计数。 在这里我们描述了测量小鼠组织的TBI和NTBI摄取的详细协议。
|
|
|