| A Novel Method to Construct Binary CRISPR Vectors for Plant Transformation by Single Round of PCR Amplification
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Author:
Date:
2021-04-05
[Abstract] CRISPR/Cas9 is an established and flexible tool for genome editing. However, most methods used to generate expression clones for the CRISPR/Cas9 are time-consuming. Hence, we have developed a one-step protocol to introduce sgRNA expression cassette(s) directly into binary vectors (Liu et al., 2020). In this approach, we have optimized the multiplex PCR to produce an overlapping PCR product in a single reaction to generate the sgRNA expression cassette. We also amplified two sgRNA expression cassettes through a single round of PCR. Then, the sgRNA expression cassette(s) is cloned into the binary vectors in a Gateway LR or Golden gate reaction. The system reported here provides a much more efficient and simpler procedure to construct expression clones for CRISPR/Cas9-mediated genome ...
[摘要] [摘要] CRISPR / Cas9是一种成熟且灵活的基因组编辑工具。但是,大多数用于生成CRISPR / Cas9表达克隆的方法都很耗时。因此,我们开发了一种将sgRNA表达盒直接引入二元载体的一步协议(Liu等人,2020年)。在这种方法中,我们优化了多重PCR,以在单个反应中产生重叠的PCR产物,从而生成sgRNA表达盒。我们还通过单轮PCR扩增了两个sgRNA表达盒。然后,在Gateway LR或Golden gate反应中将sgRNA表达盒克隆到二元载体中。本文报道的系统为构建用于CRISPR / Cas9介导的基因组编辑的表达克隆提供了更有效,更简单的程序。在此协议中,我们描述了使用此系统的详细分步说明。
[背景]乙acteria保卫针对病毒通过蛋白系统,由群集规则间隔开的短回文重复序列(CRISPR)中,CRISPR相关(CAS)蛋白质,CRISPR的RNA(crRNAs)和反式编码crRNA(tracrRNA)。现在,研究人员已经将其系统开发为用于靶向基因组编辑的关键工具。CRISPR –二元载体表达两个元素–具有靶序列的sgRNA(target-sgRNA)和Cas9蛋白–切割靶基因组区域。冯等人。(2013年)已经构建了网关载体,通过农杆菌介导的转化在植物中共表达Cas9和sgRNA ...
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| Gas Chromatography Detection Protocol of Short-chain Fatty Acids in Mice Feces
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Author:
Date:
2020-07-05
[Abstract] Short-chain fatty acids (SCFAs), which are formed mainly by bacteria fermenting undigested carbohydrates in the colon, they are based on the number of carbon atoms in the carbon chain. Organic fatty acids with less than 6 carbon atoms are called short-chain fatty acids. SCFAs are closely related to various aspects of the human body, so more and more researchers concentrate on SCFAs. This protocol describes, a direct injection gas chromatography detection method with a pretreatment method for extracting SCFA from mice feces by combining acidification. The corresponding sample limit of quantization (LOQ) and limit of detection (LOD) are 0.8-1.0 mg/L and 0.5-0.8 mg/L, respectively. The correlation coefficient of calibration curve is greater than 0.999. The recovery rate of the spiked ...
[摘要] [摘要] 短链脂肪酸(SCFAs)主要由细菌在结肠中发酵未消化的碳水化合物而形成,它们的基础是碳链中碳原子的数量。碳原子少于6个的有机脂肪酸称为短链脂肪酸。SCFAs与人体的各个方面密切相关,因此SCFAs的研究越来越多。本方案描述了一种直接进样气相色谱检测法和预处理法相结合从小鼠粪便中提取SCFA的方法。相应的定量限(LOQ)和检测限(LOD)分别为0.8-1.0 mg/L和0.5-0.8 mg/L。校准曲线的相关系数大于0.999。加标回收率为80%~102%。该方法可用于小鼠粪便中SCFAs的分析测定。因此,这是一种经济、有效、重复性好的小鼠SCFAs测定方法。
[背景]短链脂肪酸(SCFA)是调节和控制生物功能的重要分子(Siri Tarino et al.,2015)。短链脂肪酸通常指含有少于六个碳原子的挥发性有机脂肪酸(Wong等人,2006年;Marette和Jobin,2015年)。主要包括异丁酸、异丁酸、异丁酸。SCFAs主要由肠道微生物群产生,在结肠中发酵未消化的碳水化合物和膳食纤维。(Henningsson等人,2001年)。许多研究表明,支链脂肪酸来自支链氨基酸和亮氨酸(Koh等人,2016)。少量支链脂肪酸是通过发酵未消化的蛋白质产生的(Cummings and ...
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| CRISPR/Cas9-mediated ssDNA Recombineering in Corynebacterium glutamicum
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Author:
Date:
2018-10-05
[Abstract] Corynebacterium glutamicum is a versatile workhorse for industrial bioproduction of many kinds of chemicals and fuels, notably amino acids. Development of advanced genetic engineering tools is urgently demanded for systems metabolic engineering of C. glutamicum. Recently unveiled clustered regularly interspaced short palindromic repeats (CRISPR) and their CRISPR-associated proteins (Cas) are now revolutionizing genome editing. The CRISPR/Cas9 system from Streptococcus pyogenes that utilizes NGG as protospacer adjacent motif (PAM) and has good targeting specificity can be developed into a powerful tool for efficient and precise genome editing of C. glutamicum. In this protocol, we described the general procedure for CRISPR/Cas9-mediated ssDNA ...
[摘要] 谷氨酸棒杆菌是多种化学品和燃料,特别是氨基酸的工业生物生产的多功能工具。 迫切需要开发先进的基因工程工具用于 C的系统代谢工程。谷氨酸。 最近推出的聚集的有规律的间隔短回文重复序列(CRISPR)和它们的CRISPR相关蛋白(Cas)现在正在彻底改变基因组编辑。 来自 Streptococcus pyogenes 的CRISPR / Cas9系统利用NGG作为原型间隔区相邻基序(PAM)并具有良好的靶向特异性,可以开发成为 C的高效和精确基因组编辑的有力工具。谷氨酸。 在该方案中,我们描述了 C中CRISPR / Cas9介导的ssDNA重组工程的一般程序。谷氨酸。 可以在 C中引入小的修改。 谷氨酸染色体,编辑效率高达90%。
【背景】革兰氏阳性土壤细菌 Corynebacterium glutamicum 是用于氨基酸,生物燃料和聚合物构建模块的工业生物生产的多功能工具(Becker et al。,2016)。在 C工程的早期阶段。谷氨酸,随机诱变结合对氨基酸类似物的表型抗性的阳性选择是最常用的策略(Vertes et al。,2005)。 C中的遗传操作。谷氨酸(glutamicum)于1984年启动,并成为菌株改良的关键促成策略(Ozaki et al。,1984)。常规使用的基因破坏和插入 ...
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