Dot-Blot Hybridization for Detection of Five Cucurbit Viruses by Digoxigenin-Labelled cDNA Probes

Dot-blot hybridization was applied in this paper to detect five viruses infecting cucurbitaceous crops, Zuccini yellow mosaic virus （ZYMV）, Watermelon mosaic virus （WMV）, Cucumber mosaic virus （CMV）, Papaya ringspot viruswatermelon strain （PRSV-W） and Squash mosaic virus （SqMV）, as a good alternative assay in seed health test and epidemiological and transgenic research. Digoxigenin-labelled cDNA probes of the five viruses were synthesized by PCR with the specific primers and applied in dot-blot hybridization to detect five viruses in crude extraction of the infected leaves. And three SqMV probes of different lengths （0.55, 1.6, and 2.7 kb, respectively） were designed to investigate the effect of hybridization. The results showed that the sensitivity for detecting the crude extraction of infected leaves by ZYMV, WMV, CMV, PRSV-W, and SqMV was down to 1：160, 1：160, 1：320, 1：160, and 1：320, respectively. Three SqMV probes of different length showed no differences on the sensitivity and specificity. The digoxigenin-labelled probes prepared by PCR could be used for accurate and rapid identification of 5 viruses infecting cucurbitaceous crops with good stabilities, sensitivities, specificity, and reproducibilifies.

A SIMULTANEOUS MULTI-PROBE DETECTION LABEL-FREE OPTICAL-RESOLUTION PHOTOACOUSTIC MICROSCOPY TECHNIQUE BASED ON MICROCAVITY TRANSDUCER

We demonstrate the feasibility of simultancous multi-probe detection for an optcal-resolution photoacoustic microscopy(OR-PAM)system.OR-P AM has elicited the attention of biomedical imaging researchers because of its optical absorption contrast and high spatial resolution with great imaging depth.OR-PAM allows label-free and noninvasive imaging by maximizing the optical absorption of endogenous biomolecules.However,given the inadequate absoption of some biomolcules,detection sensitivity at the same incident intensity requires improvement.In this study,a modulated continuous wave with power density less than 3mW/cm^(2)(1/4 of the ANSI safety limit)excited the weak photoacoustic(PA)signals of biological cells.A microcavity traneducer is developed based on the bulk modulus of gas five orders of magnitude lower than that of solid;air pressure variation is inversely proportional to cavity volume at the same temperature increase.Considering that a PA wave expands in various directions,detecting PA signals from different positions and adding them together can increase detection sensitivity and signal-to-noise ratio.Therefore,we employ four detectors to acquire tiny PA signals simul-taneously.Experimental results show that the developed OR-PAM system allows the label-free imaging of cells with weak optical absorption.

Application and development of fluorescence probes in MINFLUX nanoscopy(invited paper)

The MINimal emission FLUXes(MINFLUX)technique in optical microscopy,widely recognized as the next innovative fluorescence microscopy method,claims a spatial resolution of 1-3 nm in both dead and living cells.To make use of the full resolution of the MINFLUX microscope,it is important to select appropriate fluorescence probes and labeling strategies,especially in living-cell imaging.This paper mainly focuses on recent applications and developments of fluorescence probes and the relevant labeling strategy for MINFLUX microscopy.Moreover,we discuss the deficiencies that need to be addressed in the future and a plan for the possible progression of MINFLUX to help investigators who have been involved in or are just starting in the field of super-resolution imaging microscopy with theoretical support.

O-GlcNAc糖基化修饰的研究进展

蛋白质的N-乙酰氨基葡萄糖(O-linked-N-acetylglucosamine,GlcNAc)修饰是一种广泛存在于真核细胞内的O-连接的单糖修饰,其通过β-糖苷键将GlcNAc与细胞质或核蛋白上的丝氨酸或苏氨酸残基结合。O-GlcNAc糖基化修饰可以调控基因的表达、调节信号转导、参与免疫保护和细胞代谢等生理过程,其异常表达与某些疾病相关,如糖尿病、癌症、心血管和神经退行性疾病等,明确蛋白质的糖基化修饰位点对阐明疾病的发生具有重要意义。由于O-GlcNAc修饰是一种动态、化学计量的修饰,质谱检测信号响应低,导致位点鉴定困难。本文将基于O-GlcNAc的生物学功能,对O-GlcNAc糖蛋白的富集方法进行归纳总结,为未来O-GlcNAc相关研究提供思路。

负载荧光探针的指示标签对三文鱼新鲜度的实时可视化监测

实时可视化监测鱼肉新鲜度,对于保障食品质量和消费者安全至关重要。以二甲氨基肉桂醛和异弗尔酮丙二腈为原料,合成一种具有供体(D)-π-受体(A)结构的荧光探针CDI,用来实时监测三文鱼肉的新鲜度。此探针对13种胺类物质响应明显,且对水产品腐败过程中产生的尸胺的荧光检测限低至9.91μmol/L。采用物理沉降法将探针CDI负载到纤维滤纸上,再加入盐酸使其质子化,得到负载探针CDI+H~+的指示标签。将指示标签置于三文鱼肉上空时,随着三文鱼肉新鲜度的下降,指示标签从白色变为浅黄色直至黄色,荧光逐渐开启,从紫粉色变为橙红色。通过对照总挥发性盐基氮值,验证了负载探针CDI+H^(+)的指示标签可以通过比色荧光双响应信号很好地区分三文鱼肉的3个新鲜度等级。

The LB Films of Dansyl Chloride Labeled Octadecylamine and Its Fluorescence Lifetime

Octadecylamine was derivatized with dansyl chloride (5-dimethylaminonaphthalene-1-sulfonyl chloride) In order to simplify and understand the LB films of fluorescent probe labeling proteins. its monolayer and multilayers in the absence and presence of stearic acid were deposited by LB technique. Fluorescence spectra and lifetimes of the fluorescent products were studied to elucidate the microenvironment of molecules in the LB films.

Evaluation of a sulfonated DNA probe (sulfoprobe) for diagnosis of falciparum malaria

In this study,the DNA probe pPF14 was nonradioactively labelled by sulfo-modifica-tion,and used in a dot blot hybridization assay for detection of P.falciparum.The resultsshowed that the sulfoprobe successfully detected 25pg purified DNA and 0.001% parasitemia ofcultured P.falciparum,and did not react with human leukocyte DNA.In the study of 179clinical blood samples of malaria patients from Yunnan province,the DNA probe results corre-lated well with blood smear ones.Of 107 P.falciparum samples determined by microscope ex-amination,99 were positive by sulfoprobe (92.5%);Of 72 P.vivax samples,1 was crosslyreacted;no cross reactions were found with any of 48 normal blood samples.It is indicated thatsulfoprobe may be useful in specific diagnosis and epidemiological investigation of P.falciparuminfection.

DETECTION OF STRAND BREAKS OF DNA IN HUMAN EARLY CHORIONIC VILLUS CELLS INDUCED BY DIAGNOSTIC ULTRASOUND USING ^(32)P-LABELED ALU HYBRIDIZATION

Objective To explore if strand breaks of DNA in human early chorionic villus cells in uterus were induced by diagnostic ultrasound and to evaluate the method used for detection of single-stranded breaks and double-stranded breaks in human DNA. Methods 60 normal pregnant women aged 20-30, who underwent artificial abortion during 6-8 weeks of gestation, were randomly divided into 2 experimental groups: All 30 cases were exposed to diagnostic ultrasound in uterus for 10 minutes, and 24 hours later chorionic villi were extracted; the other 30 cases were taken as the control group. Single-stranded DNA and double-stranded DNA in villus cells in all cases were isolated by the alkaline unwinding combined with hydroxylapatite chromatography, and were quantitatively detected using 32 P-labeled Alu probe for dot-blotting hybridization. Results There was no significant difference in quantity and percentage in single-stranded DNA and double-stranded DNA between 2 groups (P>0.05). 32 P-Alu probe could only hybridize with human DNA, and could detect DNA isolated from as few as 2.5×10 3 chorionic villus cells and 0.45ng DNA in human leukocytes. Conclusion The results suggested that there were no DNA strand damages in human chorionic villus cells when the uterus was exposed to diagnostic ultrasound for 10 minutes. The method,^(32)P-Alu probe for dot-blotting hybridization, was even more specific, sensitive and accurate than conventional approaches.

免疫层析试纸条在食品安全检测中的应用

免疫层析试纸条检测技术融合免疫技术和层析技术,具有制作简单、成本低、检测快速等优点,在食品安全检测领域应用广泛。阐述了免疫层析试纸条的基本原理。简要介绍了免疫层析试纸条的标记探针。综述了免疫层析试纸条在农兽药残留、重金属、食品添加剂、违禁食品添加物质、生物毒素、食源性致病菌和人畜共患病等检测中的应用。

几种动物肉源性成分膜芯片检测方法的建立

用斑点杂交技术构建对牛、羊、鸭肉源性成分快速检测的膜芯片方法。在3种动物的线粒体细胞色素b基因上设计特异性引物,对3种动物基因组进行PCR扩增,扩增产物用地高辛进行标记,作为标记探针。将3种动物PCR扩增产物固定到尼龙膜上,再选取3种常见动物作为参照,将其扩增产物一并固定到尼龙膜上。将制作好的膜芯片与标记探针进行斑点杂交试验,来检验标记探针的标记效率和特异性。试验结果表明,标记探针在1 pg/μL浓度下显点清晰可见;3种标记探针分别与6种动物源性扩增产物杂交,结果标记探针只与其对应扩增源性产物发生显点。证明研究设计的膜芯片标记探针具有灵敏度高、特异性强的特点,符合膜芯片检测要求,从而成功构建了一种快速检测牛、羊、鸭3种动物肉源性的膜芯片方法,同时也为动物源性成分检测提供新的依据。

荧光标记技术在新型农用化合物创制中的应用现状及进展

荧光标记技术广泛应用于现代社会的各个方面,但其在农用化合物创制领域的应用鲜见综述。基于近10 a国内外农用化合物创制领域的荧光标记技术相关文献,系统总结了荧光标记技术中荧光染料的种类,综合介绍了荧光探针技术和免疫荧光技术在新型农用化合物创制领域的应用现状及进展,分析了目前荧光标记技术在新型农用化合物创制领域存在的局限与不足,并对未来荧光标记技术的发展趋势进行了展望。

多重实时荧光PCR TaqMan-MGB杂交探针标记法快速鉴定转基因玉米MIR162

为对转基因玉米MIR162的进口实行监测、规范转基因玉米在国内市场中的流通,建立一种转基因玉米MIR162准确快速的检测方法,通过设计转基因玉米MIR162品系特异性序列的引物和探针,摸索和优化多重荧光PCR体系和参数,开发建立多重实时荧光PCR TaqMan-MGB杂交探针标记法快速鉴定转基因玉米MIR162。结果表明,转基因玉米MIR162品系标准品和平行样品中内标基因和品系特异性基因均出现明显扩增曲线,其他转基因玉米品系标准品仅内标基因有扩增曲线,空白对照无扩增曲线,说明该TaqMan-MGB探针对转基因玉米MIR162品系具有扩增特异性。该方法可作为鉴定筛查转基因玉米MIR162品系及其转化体成分的有效方法,用于规范管理转基因产品在市场上的流通。

Intracellular RNA Labeling Technologies for the Analysis of RNA Biology

As a cornerstone of the central dogma of molecular biology,RNA plays vital roles in living organisms.Over the past few decades,many RNA labeling technologies have been developed to elucidate the biological function of RNA.These technologies have signifi-cantly advanced our understanding of RNA secondary structure,localization,and turnover.Additionally,taking advantage of these innovative RNA labeling approaches,plenty of tool kits have been devised for the regulation of RNA-related biological process,such as gene expression and gene editing.In this review,we primarily focus on an array of intracellular RNA labeling methods,encom-passing chemical probes-based labeling,metabolic labeling,and proximity-dependent labeling.We also provide a brief overview of their applications in the research of RNA biology.Finally,the perspectives of RNA labeling are also discussed.

HER2靶向放射性分子影像探针的研究进展

人表皮生长因子受体2(HER2)在大约20%的乳腺癌患者中过度表达,是乳腺癌治疗的一个重要分子靶点.HER2靶向治疗的重要前提是对肿瘤HER2表达的精确测定.利用HER2靶向放射性分子影像探针的核医学影像是检测HER2表达情况的重要手段.它能够在诊疗过程中对肿瘤HER2表达进行可重复的全面评估,同时它解决了乳腺癌的异质性以及取样困难等传统方法存在的问题.目前,多种HER2靶向的分子影像探针(单克隆抗体、抗体片段、纳米抗体、亲和体、多肽)正处于临床前和早期临床研究中.文章综述了靶向HER2的抗体和多肽类放射性分子探针在核医学分子影像中的研究进展,指出用其进行临床转化时所面临的挑战,为开发新的HER2靶向分子影像探针提供思路.

Preparation of Digoxigenin labelled Probe and Detection of HBV DNA in Liver and Extrabepatic Tissue with in Situ Hybridization

A new rapid technique for intrahepatic and extrahepatic HBV DNA detection by using digoxigenin labelled probe with in situ hybridization was developed.This technique has the advantage of being non-radioactive and a quick procedure yielding stable results and showing a clear background.

二茂铁标记DNA电化学探针的研制及性质研究

以乙基 -( 3-二甲基丙基 )碳化二亚胺盐酸盐 ( EDC)为偶联活化剂 ,利用缩合反应分别将电化学活性物质氨基二茂铁 ( Aminoferrocene,AFC)和醛基二茂铁 ( Ferrocenecarboxaldehyde,FCA)成功地标记在变性小牛胸腺 DNA片段上 ,制备成二茂铁标记 DNA探针 .分别采用电化学、紫外、红外光谱等方法研究了二茂铁标记 DNA探针的性质 ,计算了二茂铁的标记效率 ,变性小牛胸腺 DNA的反应效率以及二茂铁化合物与变性小牛胸腺 DNA的反应比率 .实验表明 ,氨基二茂铁和醛基二茂铁与 DNA上的磷酸基是以 1∶ 1比率进行的反应 ,该标记反应不影响 DNA链碱基的紫外吸收 ,二茂铁标记 DNA探针在石墨电极上有良好的电化学响应 .将制备好的二茂铁标记 DNA电化学探针置于冰箱中冷冻 (温度低于 -1 5℃ )保存 3个月后用于测定 ,峰电流仅下降 1 .

荧光染料探针分子对变异细胞的识别

介绍了变异细胞的结构特征、细胞识别与荧光标记技术以及荧光染料探针分子标记细胞的方式。简述了荧光染料探针分子用于变异细胞组织的标记与识别的研究新进展。并针对目前荧光染料探针分子的应用现状,分析了未来的发展趋势,包括增强荧光染料探针分子与人体组织的相容性、靶向性,提高其灵敏度,降低毒性等的方法和途径。简述了固相合成分离技术用于探针分子的制备与纯化的优越性。

一种新的荧光素类荧光探针的设计合成及其对血清中组氨酸的选择性标记

The synthesis of a novel long-wavelength fluorescent probe, 3-epoxypropoxy fluorescein, and its properties for labeling of histidine are briefly described in this communication. The probe is highly selective for histidine, and other amino acids with a concentration of 1 000 times higher than that of histidine did not show noticeable interferences. As an application of this probe, fluorescent labeling of histidine in human serum was attempted and the obtained results were in agreement with those given by using histidine-nickel complex adsorptive voltammetry, both of which were within the normal range of the results reported in literatures.

地高辛标记探针检测猪胸膜肺炎放线杆菌的研究与应用

利用PCR反应扩增出胸膜肺炎放线杆菌ApxⅣ基因650 bp的DNA,回收并纯化PCR产物,用地高辛标记,制备出地高辛标记的核酸探针。该探针与不同血清型的胸膜肺炎放线杆菌均能发生特异性杂交,而与大肠杆菌、多杀性巴氏杆菌、沙门氏菌、葡萄球菌、猪肺炎支原体、支气管败血波氏杆菌等细菌的核酸杂交均为阴性。对胸膜肺炎放线杆菌的最低检出限量为10×102 个放线杆菌。对疑似胸膜肺炎放线杆菌感染病变组织检测结果表明,在扁桃体、鼻腔、气管、肺脏均可检测出胸膜肺炎放线杆菌,以扁桃体的检出率最高。为猪胸膜肺炎放线杆菌的诊断和流行病学调查提供了良好的方法。