Analysis of DNA Sequencing Reaction Products Made with 7-Halo-7-deaza-2′-deoxyguanosine-5′-triphosphate

Abstract

7-Chloro- and 7- Iodo-7-Deaza-2′-Deoxyguanosine-5′-Triphosphates were employed as substrates replacing dGTP, dITP, or 7-Deaza-2′-Deoxyguanosine-5′-Triphosphate in sequencing reactions with Thermo Sequenase^TM. Analysis of the reaction products by denaturing gel electrophoresis indicates DNA containing these halogenated analogs can form strong secondary structures.     

腺相关病毒载体工程毒株精细化纯化

[背景] 大量制备高纯度的重组腺相关病毒（Recombinant Adeno-Associated Virus,rAAV）,是以腺相关病毒（AAV）为投递载体的基因靶向治疗或基因工程药物研发过程中需要解决的重要问题。[目的] 利用层析柱法大量纯化质粒和rAAV细胞培养液,以获得高纯度的rAAV颗粒。[方法] 对组装rAAV的3种质粒用HiPrep^TM10 Sepharose 6FF和HiTrap PlasmidSelect Xtra凝胶层析柱纯化,目的是得到组装AAV的超螺旋质粒DNA,然后对组装rAAV过程中的AAV-293细胞培养方法进行优化,组装成功病毒后,再对收集到的细胞提取液用HiLoad^TM10Q和HiLoad^TM10SP阴阳离子交换层析柱纯化,最后用纯化浓缩后的rAAV感染HT1080细胞,通过流式细胞仪检测荧光表达细胞数,计算浓缩后活病毒感染滴度。[结果] HiPrep和HiTrap层析柱纯化后得到大量高纯度的超螺旋质粒DNA,组装病毒后,用HiLoad柱纯化获得大量高纯度的rAAV颗粒,通过测定,rAAV基因组滴度达到（2.46±0.37）×10¹² TCID₅₀/mL （MOI=1.0×10⁴）。[结论] 通过一系列精细化组装纯化制备出高纯度、高滴度rAAV病毒颗粒。     

抗菌肽AD基因的合成

设计并合成了一种新型抗菌肽基因,合成的抗菌肽(cecropin)AD基因全长140个碱基对,克隆于pCR^TM2.1载体上,经DNA序列分析证实,合成的cecropin AD基因的碱基序列与设计序列完全一致.     

Improving Indel Detection Specificity of the Ion Torrent PGM Benchtop Sequencer

The emergence of benchtop sequencers has made clinical genetic testing using next-generation sequencing more feasible. Ion Torrent''s PGM^TM is one such benchtop sequencer that shows clinical promise in detecting single nucleotide variations (SNVs) and microindel variations (indels). However, the large number of false positive indels caused by the high frequency of homopolymer sequencing errors has impeded PGM^TM''s usage for clinical genetic testing. An extensive analysis of PGM^TM data from the sequencing reads of the well-characterized genome of the Escherichia coli DH10B strain and sequences of the BRCA1 and BRCA2 genes from six germline samples was done. Three commonly used variant detection tools, SAMtools, Dindel, and GATK''s Unified Genotyper, all had substantial false positive rates for indels. By incorporating filters on two major measures we could dramatically improve false positive rates without sacrificing sensitivity. The two measures were: B-Allele Frequency (BAF) and VARiation of the Width of gaps and inserts (VARW) per indel position. A BAF threshold applied to indels detected by UnifiedGenotyper removed ∼99% of the indel errors detected in both the DH10B and BRCA sequences. The optimum BAF threshold for BRCA sequences was determined by requiring 100% detection sensitivity and minimum false discovery rate, using variants detected from Sanger sequencing as reference. This resulted in 15 indel errors remaining, of which 7 indel errors were removed by selecting a VARW threshold of zero. VARW specific errors increased in frequency with higher read depth in the BRCA datasets, suggesting that homopolymer-associated indel errors cannot be reduced by increasing the depth of coverage. Thus, using a VARW threshold is likely to be important in reducing indel errors from data with higher coverage. In conclusion, BAF and VARW thresholds provide simple and effective filtering criteria that can improve the specificity of indel detection in PGM^TM data without compromising sensitivity.     

A Novel and Convenient Method for the Synthesis of Free 5′-Thiol Modified Oligonucleotides

Abstract

The synthesis of free 5′-thiol-modified oligonucleotides using a 4,4′,4″-trimethoxytrityl (TMTr)-protected linker and standard Poly-Pak^TM purification has been described.     

Cloning and Sequence Analysis of a cDNA from Seminal Vesicle Tissue Encoding the Precursor of the Major Protein of Bull Semen

Abstract

A cDNA library derived from poly(A)⁺RNA of bull seminal vesicle- tissue was screened with a synthetic DNA hybridisation probe specific for the major protein of bull semen. A positive clone pMP17, containing a 680 bp insert, was sequenced. In combination with primer extension sequencing of poly(A)⁺RNA, a DNA sequence of 700 bp was determined. This DNA encoded a reading frame for 134 amino acids, starting with an ATG and terminated by a TAG codon. This comprised 25 amino acids of a signal peptide followed by 109 amino acids with the known sequence of the major protein.     

Comparative study of chemical pathology sample collection tubes at the largest hospital in South Africa

BackgroundBarricor^TM Lithium heparin plasma tubes are new blood tubes that have been introduced to overcome the effects of gel in serum separator tubes (SST) and the shortcomings of standard Lithium heparin plasma. We aimed to evaluate Barricor^TM tubes as an alternative to serum separator tubes and compare the stability between the tubes.MethodsForty-four paired samples were collected using both Barricor^TM and SST. We compared five analytes at baseline (<6 h) and after every 24 h using the PassingBablok and Bland-Altman plots. Aspartate aminotransferase (AST), potassium (K), phosphate (PO4) , lactate dehydrogenase (LDH), and creatinine were analysed in both tubes. We calculated the percentage difference for each analyte between the baseline and time intervals to assess analyte stability. The percentage difference was compared to the desirable specification for bias and reference change value (RCV).ResultsAll analytes were comparable at baseline. Statistical differences (p<0.001) became evident after 24 h. PO4, K, and creatinine had a mean difference that exceeded the desirable specification for bias (-9.59%, - 9.35%, and -4.59%, respectively). Potassium was stable up to 24 h in both tubes. LDH showed better stability in SST (144 h vs 96 h). PO4 concentrations were more stable in both tubes with the SST (96 h vs 72 h). Creatinine and AST had the longest stability in both tubes compared to other analytes (144 h).ConclusionsData demonstrated variability and similarities in analyte concentrations and stability, respectively, in both tubes.     

Enzymatic synthesis of cetyl oleate in a solvent-free medium using microwave irradiation and physicochemical evaluation

Abstract

A cosmetic ester, cetyl oleate was synthesized using microwave irradiated system. The esterification reaction was carried using Candida antarctica lipase B in a solvent-free media. The influence of various reaction parameters was studied, and the efficiency of Fermase CALB^TM10000 was compared with other enzymes. Equilibrium conversion of 97.5% was obtained within 20?min at 60?°C temperature, 1:2 oleic acid to cetyl alcohol molar ratio and 4% w/w dose of lipase. A comparative study showed that microwave irradiation is a much more efficient method than ultrasound irradiation and conventional heating. Fermase CALB^TM10000 was reusable over 6 enzymatic cycles as its stability improved under microwave system. Physicochemical parameters of cetyl oleate were tested in order to analyze its suitability for further cosmetic use.     

Characterization of aerobic heterotrophic bacteria in cold and nutrient-poor freshwater ecosystems

Aerobic heterotrophic bacteria present in the surface water of three cold and nutrient-poor lakes in the Chilean Patagonia (Alto Reino, Las Dos Torres and Venus) were analysed for genetic similarity and metabolic diversity using 16S ribosomal DNA and the Biolog EcoPlate^TM system, respectively. Bacterial fingerprints of water samples in enriched and non-enriched nutrient broth demonstrated a >50% fingerprinting similarity between the lakes. Metabolic activity was also similar. However, the Biolog EcoPlate^TM system carbon substrates revealed functional diversity. Lake Las Dos Torres showed the most fingerprinting similarity between enriched and non-enriched cold water samples. The amounts of living and viable bacteria were also higher in this lake’s water sample, suggesting a predominance of facultative oligotrophic groups. DNA sequencing analysis demonstrated the presence of phylum Bacteroidetes in Lake Alto Reino; phyla Bacteroidetes and Gammaproteobacteria in Lake Las Dos Torres; and phyla Bacteroidetes, Alphaproteobacteria, and Gammaproteobacteria in Lake Venus. Although each lake had a unique bacterial community structure, the different bacterial groups may be performing similar metabolic functions, given the similarity in extreme environmental conditions.     

不同DNA聚合酶对运用ARTIC工作流的新型冠状病毒纳米孔测序的影响

摘要 目的：为了验证不同高保真DNA聚合酶是否会对运用ARTIC工作流进行新型冠状病毒纳米孔测序产生影响。方法：使用英国Nanopore公司MinION测序仪对2份已获得全基因组序列的新冠肺炎确诊病例核酸样本分别采用KAPA HiFi HotStart ReadyMix,PrimeSTAR?誖GXL DNA Polymerase和NEBNext High-Fidelity 2X PCR Master Mix进行ARTIC工作流的多重PCR扩增,对扩增产物进行测序,并对测序质量进行分析。结果：不同高保真DNA聚合酶在相同扩增条件下,扩增产物的质检结果和测序质量均不相同,NEBNext High-Fidelity 2X PCR Master Mix在覆盖度和测序深度上明显好于另外两种酶。结论：NEBNext High-Fidelity 2X PCR Master Mix在纳米孔新型冠状病毒ARTIC快速测序工作流中的应用效果较好。     

7-Deaza-2′-deoxyinosine: A Stable Nucleoside with the Ambiguous Base Pairing Properties of 2′-Deoxyinosine

Abstract

The base pairing ambiguity of 7-deaza-2′-deoxyinosine (c⁷I_d, 2) was studied and was found to be the same as that of 2′-deoxyinosine. The duplex stability decreases in the order [d(c⁷I-C) > d(c⁷I-A) > d(c⁷I-T) > d(c⁷I-G)]. Modified nucleosides were used to probe the various base pair motifs which were the same for dl and c⁷I_d. The 7-deazapurine nucleoside (2) is extremely stable against acid or base. As oligonucleotides can be prepared using phosphoramidite chemistry and DNA is accessible by enzymic polymerisation of the triphosphate of 2, the latter can be used as an universal nucleoside for the sequencing of DNA by chemical degradation and is otherwise a facile substitute of 2′-deoxyinosine when stability in acidic or alkaline solution is required.     

循环肿瘤DNA突变检测方法研究进展

循环肿瘤DNA(Circulating Tumor DNA,ctDNA)含有肿瘤的遗传信息,与肿瘤组织具有高度的一致性,可代替肿瘤组织用于肿瘤的早期诊断,预后监测和药物疗效监测,是一种具有良好临床应用前景的液体活检标记物。但血液中的ctDNA片段化程度高,含量稀少,且与野生型DNA混合存在(约1%甚至更低),并会随着患者肿瘤分期等情况动态变化,造成了ctDNA检测困难,需要高灵敏度高特异性的突变检测方法,才能够从大量的野生型DNA中检测出微量突变型ctDNA。目前,灵敏度和特异性能够满足ctDNA检测需求的方法主要有扩增阻滞突变系统PCR(Amplification Refractory Mutation System PCR,ARMS-PCR)、钳制PCR(Clamping-PCR)、数字化PCR(Digital-PCR)、西格诺公司的质谱分辨技术(Sequenom UltraseekTM)和高通量测序技术。本文对这些方法的原理、特点、最新进展和应用前景进行了综述,为研究人员选择合适的ctDNA检测方法提供理论依据。     

New insights into the QuikChangeTM process guide the use of Phusion DNA polymerase for site-directed mutagenesis

The QuikChange^TM site-directed mutagenesis method is popular but imperfect. An improvement by using partially overlapping primers has been reported several times; however, it is incompatible with the proposed mechanism. The QuikChange^TM method using complementary primers is proposed to linearly amplify a target plasmid with the products annealing to produce double-stranded DNA molecules with 5′-overhangs. The overhang annealing is supposed to form circular plasmids with staggered breaks, which can be repaired in Escherichia coli after transformation. Here, we demonstrated that the PCR enzyme fills the 5′-overhangs in the early cycles, and the product is then used as the template for exponential amplification. The linear DNA molecules with homologous ends are joined to generate the plasmid with the desired mutations through homologous recombination in E. coli. The correct understanding is important to method improvements, guiding us to use partially overlapping primers and Phusion DNA polymerase for site-directed mutagenesis. Phusion did not amplify a plasmid with complementary primers but used partially overlapping primers to amplify the plasmid, producing linear DNA molecules with homologous ends for site-directed mutagenesis.     

Sequencing of Synthetic DNA Fragments Containing Various 5-Substituted Pyrimidines by Solid-Phase Chemical Degradation Using CCS Paper

Abstract

It is reported on solid-phase chemical degradation sequencing of lore than 50 synthetic DNA fragments containing various 5-substituted pyrimidines including uracil (U), 5-fluorouracil (F⁵U), 5-bromouracil (Br⁵U), α and β anomers of 5-propyluracil (α-prop⁵U and B-prop⁵U) and 5-methylcytosine (a⁵C), Characteristic sequence patterns of oligonucleotides containing these base analogues are presented and their modification behaviour discussed     

Combined multimodal ctDNA analysis and radiological imaging for tumor surveillance in Non-small cell lung cancer

BackgroundRadiology is the current standard for monitoring treatment responses in lung cancer. Limited sensitivity, exposure to ionizing radiations and related sequelae constitute some of its major limitation. Non-invasive and highly sensitive methods for early detection of treatment failures and resistance-associated disease progression would have additional clinical utility.MethodsWe analyzed serially collected plasma and paired tumor samples from lung cancer patients (61 with stage IV, 48 with stages I-III disease) and 61 healthy samples by means of next-generation sequencing, radiological imaging and droplet digital polymerase chain reaction (ddPCR) mutation and methylation assays.ResultsA 62% variant concordance between tumor-reported and circulating-free DNA (cfDNA) sequencing was observed between baseline liquid and tissue biopsies in stage IV patients. Interestingly, ctDNA sequencing allowed for the identification of resistance-mediating p.T790M mutations in baseline plasma samples for which no such mutation was observed in the corresponding tissue. Serial circulating tumor DNA (ctDNA) mutation analysis by means of ddPCR revealed a general decrease in ctDNA loads between baseline and first reassessment. Additionally, serial ctDNA analyses only recapitulated computed tomography (CT) -monitored tumor dynamics of some, but not all lesions within the same patient. To complement ctDNA variant analysis we devised a ctDNA methylation assay (^methcfDNA) based on methylation-sensitive restriction enzymes. cfDNA methylation showed and area under the curve (AUC) of > 0.90 in early and late stage cases. A decrease in ^methcfDNA between baseline and first reassessment was reflected by a decrease in CT-derive tumor surface area, irrespective of tumor mutational status.ConclusionTaken together, our data support the use of cfDNA sequencing for unbiased characterization of the molecular tumor architecture, highlights the impact of tumor architectural heterogeneity on ctDNA-based tumor surveillance and the added value of complementary approaches such as cfDNA methylation for early detection and monitoring     

二代测序应用于检测GT1-7细胞中KISS1和GnRH启动子的DNA甲基化状态的研究

目的:利用二代测序技术检测GT1-7细胞中KISS1和GnRH基因启动子范围内的甲基化状态,并用金标准的亚硫酸氢盐修饰后的克隆测序作为对照,比较二代测序与金标准克隆测序在研究DNA甲基化检测中的差别。方法:提取GT1-7细胞基因组DNA并进行亚硫酸氢盐处理。进行巢式PCR,将PCR产物进行二代测序。同时采用金标准的亚硫酸氢盐修饰后克隆测序的方法作为对照,对相同批次的PCR产物进行克隆测序。结果:PCR产物二代测序结果表明KISS1和GnRH两个基因的27个CpG甲基化位点信息完整,结果准确。挑取10个克隆进行一代测序结果表明序列无丢失,KISS1和GnRH两个基因的27个CpG甲基化位点信息完整。结论:利用高通量的二代测序技术能够有效的对DNA甲基化的PCR产物进行检测,二代测序和克隆测序都是研究DNA甲基化的有效方法,但前者与克隆测序相比每一个读取序列(reads)都相当于一个单克隆,且二代测序每个区段得到成百上千个reads,因此二代测序结果更加精确。