实时荧光定量PCR法检测外源性DNA在重组Ⅲ型人源化胶原蛋白冻干纤维中的残留

目的对实时荧光定量PCR(qPCR)法检测重组Ⅲ型人源化胶原蛋白冻干纤维中的外源性DNA残留量进行探究和分析,确定该方法用于DNA质量控制的可行性。方法采用宿主细胞残留DNA样本前处理试剂盒(磁珠法)提取DNA,利用E.coli残留DNA检测试剂盒(PCR-荧光探针法)进行扩增反应,绘制标准曲线,建立重组Ⅲ型人源化胶原蛋白冻干纤维中外源性DNA残留量的qPCR检测方法。结果对8批重组Ⅲ型人源化胶原蛋白冻干纤维进行测定,外源性DNA残留量在0.03~300 pg/μl内,重复性良好,均远低于每剂10 ng,线性良好(R^(2)>0.99),回收率均在50%~150%之间。结论该方法可用于重组Ⅲ型人源化胶原蛋白冻干纤维中外源性DNA残留量的定量测定。

东方蜜蜂微孢子虫DNA拓扑异构酶Ⅲ的分子特性与系统进化分析

利用相关生物信息学软件对东方蜜蜂微孢子虫(Nosema ceranae)的DNA拓扑异构酶3(DTⅢ)进行了理化性质、分子特性、保守基序、结构域和系统进化的分析。结果表明:DTⅢ包含805个氨基酸,分子式为C4267 H6719 N1117 O1240 S34,分子质量约为94.60 ku,脂溶系数为81.84,等电点为9.08,平均亲水系数为-0.595,亲水氨基酸多于疏水氨基酸,不含典型信号肽;含有41个丝氨酸磷酸化位点,23个酪氨酸磷酸化位点及14个苏氨酸磷酸化位点;包含310个α⁃螺旋,117个β⁃折叠,37个β⁃转角及341个无规则卷曲;可同时定位于细胞核、细胞质和线粒体;东方蜜蜂微孢子虫与其他10种微孢子虫的DTⅢ均含有5个相同的保守基序(Motif 1、Motif 2、Motif 3、Motif 4和Motif 5)和2个相同的结构域(Toprim和Topoisom_bac);通过Mega 11.0软件构建东方蜜蜂微孢子虫和其他物种的DTⅢ的系统进化树,结果显示东方蜜蜂微孢子虫与绒鳌蟹肝孢虫(Hepato⁃spora eriocheir)的DTⅢ聚为一支,进化距离最近。研究结果明确了东方蜜蜂微孢子虫DTⅢ的理化性质和分子特性,并揭示东方蜜蜂微孢子虫与绒鳌蟹肠孢虫的DTⅢ亲缘关系最近,DTⅢ在东方蜜蜂微孢子虫和其他微孢子虫中具有较高的保守性。

THE ANTICANCER EFFECT AND ANTI－DNA TOPOISOMERASE II EFFECT OF EXTRACTS OF CAMELLIA PTILOPHYLLA CHANG AND CAMELLIA SINENSIS

The cytotoxic effect of extract of camellia ptilophyllachang(ECPC) and extract of camellia sinensis(ECS) onHeLa cell line, poorly differentiated nasopharyngealcarcinoma cell line(CNE2) and gastric cancer cell line(MGC-803 ) in vitro was studied using MIT assay method.The results showed that ECPC and ECS possessed significantcytotoxic effect on above three cell lines. The anticancer testin mice showed that ECPC had marked inhibitory effectagainst Ehrlich solid carcinoma(ESC) with inhibition ratesof 17. 8 48. 3% and with inhibition rates of 28. 3-54. 5% against reticular cell sarcoma(L2), and that ECShad inhibition rates of 31 . 5 -49. 4 % against ESC and 35. 8- 50% against L2. These two extracts had only marginalinhibitory effect against sarcoma- 180. The unknottingactivity of DNA topoisomerase II was inhibited completelyby ECPC and ECS at the concentration of 50 μg/ mlsuggesting that DNA topoisomerase II might be a targetenzyme of these two extracts.

EFFECT OF ACTIVE COMPOUNDS ISOLATED FROM PTERIS SEMIPINNATA L ON DNA TOPOISOMERASES AND TYROSINE PROTEIN KINASE AND EXPRESSION OF C-MYC IN LUNG ADENOCARCINOMA CELLS

Objective: To study the effect of active compound 6F and A from Pteris semipinnata L.(PsL) on the activities of DNA topoisomerase (TOPO) I and II, activities of cytosolic and membrane TPK, and expression of oncogene c-myc in lung adenocarcinoma cells. Methods: The effect of compound 6F and A on activities of cytosolic and membrane TPK was measured by scintillation counting; the effect of compound A on expression of oncogene c-myc was determined by flow cytometry indirect fluorimetry. Results: compound 6F and A could inhibit the activities of TOPO I, and they strongly inhibited the TOPO II in 0.01 mg/L and 10.0 mg/L respectively. Compound A slightly inhibited the activities of membrane TPK, but not the cytosolic one. Compound A could inhibit the expression of oncogene c-myc. Conclusion: Topoisomerases are target of compound 6F and A. Compound A could slightly inhibit the activities of TPK, and showed an inhibitory effect on the expression of oncogene c-myc.

Narciclasine,a novel topoisomerase I inhibitor,exhibited potent anti-cancer activity against cancer cells

DNA topoisomerases are essential nuclear enzymes in correcting topological DNA errors and maintaining DNA integrity.Topoisomerase inhibitors are a significant class of cancer chemotherapeutics with a definite curative effect.Natural products are a rich source of lead compounds for drug discovery,including anti-tumor drugs.In this study,we found that narciclasine(NCS),an amaryllidaceae alkaloid,is a novel inhibitor of topoisomerase I(topo I).Our data demonstrated that NCS inhibited topo I activity and reversed its unwinding effect on p-HOT DNA substrate.However,it had no obvious effect on topo II activity.The molecular mechanism of NCS inhibited topo I showed that NCS did not stabilize topo-DNA covalent complexes in cells,indicating that NCS is not a topo I poison.A blind docking result showed that NCS could bind to topo I,suggesting that NCS might be a topo I suppressor.Additionally,NCS exhibited a potent anti-proliferation effect in various cancer cells.NCS arrested the cell cycle at G_(2)/M phase and induced cell apoptosis.Our study reveals the antitumor mechanisms of NCS and provides a good foundation for the development of anti-cancer drugs based on topo I inhibition.

EFFECT OF ANTITUMOR DRUGS ON THE ACTIVITY OF DNA TOPOISOMERASE I

The activity of DNA topoisomerase Ⅱ prepared from either normal or tumor tissues were compared. It was found that the unknotting activity of the enzyme in malignant tumor cells was higher than that in normal cells. We selected some antitumor drugs including Chinese traditional medicine, and observed their effects on the unknotting activity of topoisomerase Ⅱ. The results showed that inhibition of the unknotting activity of the enzyme required very low concentrations of drugs, but much higher concentrations were required for other tested. Some antitumor drugs had no effect on the enzyme were also proved. It is interesting that carrageenan, an antiviral drug, strongly blocked the unknotting activity although its antitumor activity has not been reported.

基于电化学DNA传感器的LAMP检测方法

申请号:202410558515.7【申请日】2024.05.08【公开号】CN118127133A【公开日】2024.06.04【分类号】G01N27/26;G01N27/48;C12Q1/6844【申请人】常州先趋医疗科技有限公司【发明人】关国良;王立新;贾瑶瑶【摘要】本发明属于电化学DNA传感器检测领域,具体提供了一种基于电化学DNA传感器的LAMP检测方法,包括:电化学DNA传感器制备;通过核酸外切酶Ⅲ对LAMP产物进行预处理;通过电化学DNA传感器制备对预处理后的LAMP产物进行电信号检测。应用核酸外切酶Ⅲ对LAMP扩增产物进行处理,使得LAMP产物中靶标区域单链DNA暴露出来,增强电化学DNA传感器检测的灵敏度,整个检测过程无需洗涤,避免了复杂的操作,减少误差。

重组Ⅲ型胶原蛋白在护肤品和药械领域的应用综述

Ⅲ型胶原蛋白是一种重要的结构蛋白,广泛存在于人体的皮肤、肌腱和血管等弹性组织中,对于维持皮肤弹性、促进伤口愈合以及保持血管的完整性具有至关重要的作用。随着生物技术的发展,利用重组DNA技术在微生物或细胞中定向生产高纯度和高活性的Ⅲ型胶原蛋白的生产模式已经得到应用,不仅提高了胶原蛋白的可用性和品质,还避免了潜在的动物源传染性疾病的风险。在护肤领域,基于其优越的生物相容性和促进皮肤再生的特性,重组Ⅲ型胶原蛋白成分被广泛添加到抗衰老、保湿和修复损伤皮肤等护肤品中。在医疗器械领域,重组Ⅲ型胶原蛋白被用作生物医用材料,凭借独特的生物活性和细胞吸附特性,在促进组织再生和愈合方面展现出了巨大的应用潜力。未来,随着研究的深入和技术的进步,重组Ⅲ型胶原蛋白将在美容和医疗领域得到更广泛的应用。

钴(Ⅲ)配合物与DNA作用的研究

为了考察金属配合物中配体分子平面大小对金属配合物与DNA作用模式的影响 ,用荧光法和光度法对乙二胺合钴 (Ⅲ ) ([Co(en)3]3 +)、联吡啶合钴 (Ⅲ ) ([Co(bpy)3]3 +)和邻菲咯啉合钴 (Ⅲ ) ([Co(phen)3]3 +)与DNA的作用进行了研究。结果表明[Co(phen)3]3 +与DNA作用时除存在静电作用模式外 ,还存在插入作用 ,而[Co(en)3]3 +和[Co(bpy)3]3 +主要以静电作用与DNA结合。插入作用的强弱与配合物中配体分子平面大小有关。

Ru(Ⅲ)、Rh(Ⅲ)、Pd(Ⅱ)离子与ct-DNA的相互作用研究

本文以中药小檗碱作为分子探针,在0.01mol·L-1醋酸-醋酸钠缓冲体系中,用紫外-可见吸收及荧光光谱法研究了Ru?、Rh?、Pd?三种贵金属离子与DNA的键合相互作用。实验发现Ru?离子对小檗碱-DNA二元体系的荧光有较强的猝灭作用;而Rh?、Pd?两种离子则对该二元体系产生显著的荧光敏化作用。考察了EDTA对贵金属离子、小檗碱及DNA三元混合体系的荧光光谱的影响,初步探讨了贵金属离子与DNA可能的键合机理。

基于免标记发夹型探针和核酸外切酶Ⅲ的荧光信号放大DNA检测

设计合成了一种长臂发夹型核酸探针,结合核酸外切酶Ⅲ水解反应建立了一种免标记荧光信号放大高灵敏检测DNA的新方法。当不存在靶DNA时, SYBR Green Ⅰ荧光染料能够嵌入发夹型探针的茎部而发出很强的荧光,而当存在靶DNA并与发夹型探针杂交后,核酸外切酶Ⅲ从杂交产物的3’端开始水解发夹型探针,释放出靶DNA,并触发下一个酶水解反应,同时SYBR Green Ⅰ染料也随发夹型探针水解而释放,导致荧光信号降低,从而实现了对DNA的免标记荧光信号放大高灵敏检测。该方法的检出限低至320 fmol/L,比传统双标的分子信标的方法降低了4~5个数量级,且该方法还具有免标记、简单、快速的特点。

甲基百里酚蓝-钐(Ⅲ)配合物与鲱鱼精DNA的相互作用

在pH=7.25的Tris-HCl缓冲溶液中,以中性红(NR)作为光谱探针,采用UV光谱、FS光谱、粘度等方法研究了甲基百里酚蓝(MTB)与稀土金属离子钐[Sm(Ⅲ)]形成的配合物Sm(Ⅲ)(MTB)2与鲱鱼精DNA的作用机制.确定了Sm(Ⅲ)(MTB)2与鲱鱼精DNA之间有嵌插作用方式存在,说明Sm(Ⅲ)(MTB)2金属配合物能使鲱鱼精DNA的功能产生一定影响.

酪氨酸-钐(Ⅲ)配合物与鲱鱼精DNA的作用方式

采用UV光谱法、荧光光谱法,在pH=7.40的生理环境中用摩尔比法确定了Sm(Ⅲ)与Tyr(酪氨酸)结合的物质的量比n(Sm(Ⅲ)):n(Tyr)=1:3,Sm(Ⅲ)(Tyr)3配合物与hs(鲱鱼精)DNA结合的物质的量比n(Sm(Ⅲ)(Tyr)3):n(DNA)=3:1。用双倒数法确定了结合常数K2Θ98.15K=9.97×104L/mol和K3Θ10.15K=7.56×103L/mol。化学热力学研究显示配合物Sm(Ⅲ)(Tyr)3与hsDNA的结合过程为焓驱动;结合Scatchard法和黏度法,确定了配合物Sm(Ⅲ)(Tyr)3与hsDNA之间的作用方式为沟渠作用和嵌插作用。

光谱法研究依诺沙星与铁(Ⅲ)及其DNA的相互作用

用荧光和紫外光谱法研究了依诺沙星 (ENX)及其铁络合物与DNA的相互作用。Fe(Ⅲ )、DNA均能以静态猝灭的方式猝灭ENX分子的荧光。并且用荧光法测定了ENX -Fe(Ⅲ )和ENX -DNA二元络合物的组成和形成常数。ENX -DNA的光谱图在有Fe(Ⅲ )存在时 ,发生了明显的变化 ,表明能够形成ENX -Fe(Ⅲ ) -DNA三元络合物。研究表明在一定的浓度范围内 ,三元络合物的荧光强度与天然DNA的浓度成线性关系。讨论了反应的最佳条件。进一步探讨了依诺沙星、Fe(Ⅲ )

Nd(Ⅲ)与Hbbimp配合物的合成及其与DNA的作用研究

合成并表征了新的双核配合物 [Nd2 ( bbimp) ( CH3COO) ( CH3CH2 O) 2 ( CH3CH2 OH) ]( Cl O4 ) 2 ,Hbbimp=2 ,6-二 [二 ( 2 -苯并咪唑甲基 ) ]氨甲基 -4-甲基苯酚 .用光谱学手段研究了配合物与小牛胸腺 ( CT)DNA的作用 ,结果表明 ,配合物使 CT的 DNA最大吸收峰发生减色和红移 ;使溴化乙锭 ( EB) -DNA复合物体系荧光强度减弱 ;热变性实验表明配合物使 DNA的变性过程和降解过程共存 .在 5 0℃ ,p H=8.0时 ,单独的配合物对超螺旋质粒 p BR3 2 2 DNA的断裂的效果最好 ,可将大部分超螺旋 DNA( CCC带 )转化为缺刻产物 ( OC带 ) ;当 c( H2 O2 ) <1× 1 0 - 3mol/L ,n(配合物 )∶ n( H2 O2 ) =1∶ 2 0时 ,配合物在较低浓度时即可将CCC带全部转化为 OC带 .

光谱法研究加替沙星与Fe(Ⅲ)和DNA的相互作用

采用荧光光谱、紫外光谱法研究了加替沙星(Gatifloxacin,GTF)、Fe(Ⅲ)与DNA三元体系的相互作用。结果表明,Fe(Ⅲ)和DNA均能猝灭GTF分子的荧光。测定了GTF-Fe(Ⅲ)和GTF-DNA形成二元络合物反应的结合常数K,结合位点数n;考察了温度、溶液酸度对体系荧光强度的影响及离子干扰情况,发现DNA以静态猝灭的方式猝灭GTF-Fe(Ⅲ)体系荧光。通过离子强度和热变性DNA实验的进一步研究,揭示了加替沙星、Fe(Ⅲ)和DNA之间存在沟槽结合和静电作用。

光谱法研究洛美沙星与铁(Ⅲ)及其DNA的相互作用

用荧光和紫外光谱法研究洛美沙星(LMX)及其铁络合物与DNA的相互作用.Fe(Ⅲ)、DNA均能以静态猝灭的方式猝灭LMX分子的荧光.并且用荧光法测定了LMX-Fe(Ⅲ)和LMX-DNA二元络合物的组成和形成常数.LMX-DNA的光谱图在有Fe(Ⅲ)存在时,发生了明显的变化,表明能够形成LMX-Fe(Ⅲ)-DNA三元络合物.研究表明在一定的浓度范围内,三元络合物的荧光强度与天然DNA的浓度成线性关系.讨论反应的最佳条件.进一步证实洛美沙星、Fe(Ⅲ)和DNA的结合机理.

Sm(Ⅲ)(MTB)_2配合物与DNA作用的光谱法研究

The interaction between Sm(Ⅲ)(MTB)2 complex and Herring Sperm DNA has been studied by UV-Vis spectral, Fluorescence spectral in buffer solution of Tris-HCl (pH=7.25) using Neutral Red (NR) as a probe. The intercalation and electrostatic manner are confirmed to be the two major modes for interaction between Sm(Ⅲ)(MTB)2 complex and Herring Sperm DNA. The balance constant of Sm(Ⅲ)(MTB)2 rare earth metal complex and Herring Sperm DNA is K=4.10 × 104 L·mol-1. The results indicate that biological functions of Herring Sperm DNA are changed to a certain extend due to the interaction between Sm(Ⅲ)(MTB)2 rare earth metal complex and Herring Sperm DNA.

Salen Mn(Ⅱ)、Eu(Ⅲ)配合物抗O_2^(·-)活性及其与DNA作用的光谱性质研究

合成了5种Salen Mn(Ⅱ)及2种Salen Eu(Ⅲ)配合物。以NBT/核黄素(VB2)/蛋氨酸为O2.-的产生、检测体系,对上述配合物进行了抗O2.-活性研究,发现Mn(Ⅱ)配合物对O2.-均具有较为明显的清除活性。用荧光检测法对上述配合物与ct-DNA的作用进行了研究,结果显示其均能与DNA产生结合作用,提示具有潜在抗癌活性。

博莱霉素-Ce(Ⅲ)对DNA的切断机理初探

根据外切核酸酶Ⅲ酶解博莱霉素 Ce (Ⅲ ) [BLMA5 Ce (Ⅲ ) ]作用过的双链直线型DNA时 ,酶解速率明显增大 ,酶解产物除 5′ dAMP、 5′ dGMP、 5′ dCMP和 5′ dTMP 4种单核苷酸外 ,还有其他成分存在的实验事实 ,推测出BLMA5 Ce (Ⅲ )在DNA双链的特定部位沿 5′→ 3′的方向切断磷酸二酯键 ,使DNA的双链上形成多个暴露的 3′