应用FISH技术鉴定一个小冰麦易位系

以生物素（ｂｉｏｔｉｎ１６ｄＵＴＰ）标记的天蓝冰草（Ａｇｒｏｐｙｒｏｎｉｎｔｅｒｍｅｄｉｕｍ（Ｈｏｓｔ）Ｐ．Ｂ．＝Ｅｌｙｔｒｉｇｉａｉｎｔｅｒｍｅｄｉａ（Ｈｏｓｔ）Ｎｅｖｓｋｉ＝Ｔｈｉｎｏｐｙｒｕｍｉｎｔｅｒｍｅｄｉｕｍ（Ｈｏｓｔ）ＢａｒｋｗｏｒｔｈａｎｄＤｅｗｅｙ）染色体组ＤＮＡ为探针,普通小麦（ＴｒｉｔｉｃｕｍａｅｓｔｉｖｕｍＬ．）“中国春”ＤＮＡ为封闭,用荧光原位杂交（ＦＩＳＨ）技术对小冰麦３３号进行检测。结果表明：在一对染色体的端部显现出绿色荧光,这说明小冰麦３３号携带外源基因的冰草染色体片段位于小麦染色体端部,而且易位的染色体片段是较小的。从ＤＮＡ水平直接证明小冰麦３３是一个冰草染色体片段易位到小麦染色体端部的易位系。     

用RAPD技术鉴定两个小冰麦易位系

本文对从小冰麦异附加系中选育出的两个抗锈品系小冰麦33号,小冰麦34号及其原始亲本新曙光一号和抗源供体天兰冰草进行了RAPD分析,确定了小冰麦33号和小冰麦34号是含一段冰草DNA的易位系,文中还讨论了RAPD做为一种准确,快速鉴定易位系的方法的可行性。     

用分子原位杂交（GISH）鉴定小麦－簇毛麦双倍体、附加系、代换系和易位系

用生物素标记的簇毛麦（Ｈａｙｎａｌｄｉａｖｉｌｌｏｓａ）染色体组ＤＮＡ（ｔｏｔａｌｇｅｎｏｍｉｃＤＮＡ）作探针,以普通小麦染色体组ＤＮＡ作遮盖（用量１：２００左右）,进行有丝分裂中期和减数分裂中期Ｉ染色体的分子原位杂交（ＧＩＳＨ）,经抗生物素蛋白－辣根过氧化物酶复合物（ｂｉｏ－ｓｔｒｅｐｔａｖｉｄｉｎ－ｈｏｒｓｅｒａｄｉｓｈｐｅｒｏｘｉｄａｓｅ）和联苯胺四盐酸（ＤＡＢ）检测显色后,小麦－簇毛麦双倍体、附加系、代换系和易位系中的簇毛麦染色体及染色体片段显棕色,与显浅蓝色的小麦染色体可明显区分。用ＧＩＳＨ不仅可以检测导入小麦中的簇毛麦染色质,而且可以清楚地显示出易位染色体断裂点的确切位置。将ＧＩＳＨ用于减数分裂期染色体配对分析,还可以清晰形象地显示出同源和非同源染色体之间的配对和分离情况。     

应用G显带染色体荧光原位杂交（FISH）技术研究复杂的染色体易位

建立常规Ｇ显带染色体标本的荧光原位杂交（ＦＩＳＨ）技术,用于分析患者复杂的染色体易位。原位杂交前,用甲醛固定Ｇ显带标本,是获得良好显带和荧光杂交效果的关键步骤。仅用常规细胞遗传学方法分析,显示一例习惯性流产患者的核型为４６,ＸＸ,ｔ（１;５;１２）（１ｐｔｅｒ→１ｑ２５：：１２ｑ２４→１２ｑｔｅｒ;５ｑｔｅｒ→５ｐ１１：：１ｑ２５→１ｑｔｅｒ,１２ｐｔｅｒ→１２ｑ２４：．５ｐ１１→５ｐｔｅｒ）,而采用本方法确定患者的核型实际为４６,ＸＸ,ｔ（１;５,１２）（１ｐｔｅｒ→１ｑ２３：：１２ｑ２２→１２ｑｔｅｒ,５ｑｔｅｒ→５ｐ１１：：１ｑ２５→１ｑｔｅｒ;１２ｐｔｅｒ→１２ｑ２２：：１ｑ２３→１ｑ２５：５ｐ１１→５ｐｔｅｒ）。结果表明,新建立的Ｇ显带染色体荧光原位杂交（ＦＩＳＨ）技术能更有效地检测患者复杂的染色体易位。     

Variation of the Wheatgrass Chromosomes in Wheat-wheatgrass Disomic Addition Line TAI 14 Revealed by Fluorescence in Situ Hybridization

The karyotype of the primary wheat-wheatgrass disomic addition line TAI-14 was 2n = 44 in which all of the chromosomes were metacentric and submetacentric. However, in the progeny of the TAI-14, a pair of telocentric chromosomes were observed. In order to clarify whether the telocentric chromosomes were of common wheat or of wheatgrass, the fluorescence in situ hybridization (FISH) technique was employed. It was revealed that the wheat chromosomes exhibited red fluorescence while the ditelocentric chromosomes green fluorescence. Therefore, the primary TAI-14 was conversed from the disomic addition line into the ditelocentrie addition line. The possible explanation for such a variation and the potential significance of the ditelocentric addition line were discussed briefly.     

Characterization of Genome and Chromosomes in Octoploid Wheat wheatgrass Amphiploid Zhong 2 Using Fluorescence in situ Hybridization and Chromosome Pairing Analysis

Genomic constitution of octoploid wheat-wheatgrass amphiploid Zhong 2 was analyzed by chromosome pairing and fluorescence in sim hybridization techniques. The results indicated that the octoploid wheatwheatgrass chromosomes in Zhong 2 were derived from the distant homologous genomes of wheatgrass ( Agropyron intermedium (Host) P.B. = Elytrigia intermedia (Host) Nevski = Thinotopyrum intermedium (Host) Barkworth and Dewey, and thew distant homologous genomes were not from the E geaome of T. elongatum 2x. Zhong 2 contained 12 wheatgrass chromosomes in which a pair of chromosomes was involved in translocation between wheatgrass and wheat chromosomes.     

单体异附加系花药培养创制小麦- 中间偃麦草纯合易位系

利用单体异附加系花药培养细胞工程途径,诱导小麦与中间偃麦草发生染色体易位,通过细胞学分析、荧光原位杂交(F ISH)和SSR鉴定出纯合易位系.研究结果表明,经单体异附加系花药培养创制出1个小麦-中间偃麦草纯合易位系99-803;其花粉母细胞(PM C s)减数分裂中期I染色体构型为18.42个环状二价体 2.57个棒状二价体 0.01个单价体;中间偃麦草的7A i-1染色体与小麦7A或7B染色体发生了非罗伯逊易位,且中间偃麦草易位片段较小;通过该途径获得纯合易位系的频率约为2%.以上结果表明,单体异附加系花药培养是一条向小麦转移异源染色体小片段(基因)的快速高效途径.     

用顺序GISH-FISH 技术鉴定小麦-中间偃麦草小片段易位系

利用顺序基因组-重复序列原位杂交技术对1个来自中3不育系和普通小麦恢75杂种后代稳定株系H96276-2的染色体组成进行了分析。以中间偃麦草（Agropyronintermedium）基因组DNA为探针的荧光原位杂交结果表明,H96276-2的体细胞中有42条染色体,包括20对小麦染色体和1对小麦-中间偃麦草易位染色体,中间偃麦草染色体的易位片段位于1对小麦染色体的端部。进而用重复序列探针pSc119进行第2次荧光原位杂交,证明H96276-2中的中间偃麦草染色体易位片段位于小麦2B染色体的短臂上。     

应用荧光原位杂交和染色体配对研究八倍体小冰麦中2的染色体组构成及染色体特征

通过染色体配对分析和荧光原位杂交（ＦＩＳＨ）技术对八倍体小冰麦中２的染色体组构成进行分析,结果表明：八倍体小冰麦中２含有的冰草染色体是来自天蓝冰草（Ａｇｒｏｐｙｒｏｎ　ｉｎｔｅｒｍｅｄｉｕｍ（Ｈｏｓｔ）Ｐ．Ｂ．＝Ｅｌｙｔｒｉｇｉａ　ｉｎｔｅｒｍｅｄｉａ（Ｈｏｓｔ）Ｎｅｖｓｋｉ＝Ｔｈｉｎｏｐｙｒｕｍ　ｉｎｔｅｒｍｅｄｉｕｍ　（Ｈｏｓｔ）Ｂａｒｋｗｏｒｔｈ　ａｎｄ　Ｄｅｗｅｙ）具同亲关系的染色体组,但冰草的这种同亲关系的染色体组不同于二倍体长穗偃麦草（Ｔｈｉｎｏｐｙｒｕｍ　ｅｌｏｕｇａｔｕｍ　２Ｘ）的Ｅ组染色体。中２含有１２条冰草染色体,且有一对染色体为小麦（Ｔｒｉｔｉｃｕｍ　ａｅｓｔｉｖｕｍ　Ｌ．）染色体和冰草染色体之间易位所形成的。     

应用荧光原位杂交技术研究小冰麦异附加系TAI-14中的冰草染色体变异

对常规染色体的观察结果表明：原初的小冰麦异附加系ＴＡＩ１４为２ｎ＝４４,其中所有的染色体都是中部或近中部着丝点染色体。但在其后代中发现有一对染色体变成了端着丝点染色体。为判明变异的染色体是冰草还是小麦的染色体,用荧光原位杂交技术进行了检测,结果表明,ＴＡＩ１４中的所有小麦染色体都显示红色荧光,只有一对端着丝点染色体显示绿色荧光,说明变异的是冰草染色体,即：小冰麦异附加系ＴＡＩ１４原为二体异附加系,现变成了双端体异附加系。对变异发生的原因和双端体异附加系的用途进行了讨论。     

X染色体部分单体的母亲及相同核型的女儿

先证者,女,３３岁,１９９３年１１月１４日因外伤难免流产后３年不孕就诊。先证者２１岁结婚,婚后２年妊娠,无先兆流产,足月顺产一女婴,分娩过程正常,婴儿无窒息。２８岁第二次妊娠,约４０天不慎从山上摔下流产,行清宫术。近３年出现继发闭经,用乙芪酚、黄体酮...     

FISH methods in phycology: Phototrophic biofilm and phytoplankton applications

Abstract

Many photosynthetic microorganisms, living attached to immersed substrates or free in the water column, lack distinct morphological details, are small in size and often unculturable. Thus, whole-cell fluorescence in situ hybridization (FISH) with rRNA-targeted oligonucleotide probes has become a valuable and widely used technique to identify bacteria and protists within their natural communities. FISH methods not only allow direct, cultivation independent determination of community composition, but provide spatio-temporal quantification of microorganisms in the environment. Coupling of FISH techniques to Confocal Laser Scanning Microscopy (CLSM) has become essential for the assessment of diversity and structural integrity in three-dimensional complex biofilm samples. Combining FISH with microautoradiography (FISH-MAR) and microsensors also opens new perspectives in microbial ecology by providing new tools for revealing physiological properties of organisms with single-cell resolution. This paper briefly summarizes the application of FISH methods to phototrophic biofilm and phytoplankton research. The potential of DNA microarray technology in phycological research is highlighted, especially for the fast and accurate identification of HAB (Harmful Algal Bloom) species in marine phytoplankton. Some CLSM and FISH data from phototrophic biofilms from an Italian wastewater treatment plant are shown.     

An approach to the validation of novel molecular markers of breast cancer via TMA-based FISH scanning

Tissue microarrays (TMA) are valuable tools for validating results of array-based comparative genomic hybridization (ACGH) and other translational research applications requiring independent verification of genomic gains and losses by fluorescence in situ hybridization (FISH). However, spatial orientation and accurate manual tracking of the TMA cores is challenging and prone to error. Image analysis combined with core tracking software, implemented via an automated FISH scanning workstation, represents a new approach to FISH and TMA-based validation of novel genomic changes discovered by ACGH in breast and other cancers. Automated large-scale tissue microarray validation FISH studies of genomic gains and losses identified by ACGH for breast cancer are feasible using an automated imaging scanner and tracking/classifying software. Furthermore, by leveraging the bifunctional fluorescent and chromogenic properties of the alkaline phosphatase chromogen fast red K and combining the technology with FISH, correlative and simultaneous phenotype/genotype studies may be enabled.     

CD138免疫磁珠细胞分选的FISH技术在多发性骨髓瘤诊断中的应用

为了分析CD138免疫磁珠细胞分选的染色体荧光原位杂交(FISH)技术在提高多发性骨髓瘤(MM)细胞遗传学异常检测敏感性的作用。本研究选取我院收治的30例确诊MM的患者为研究对象,分离骨髓单个核细胞,应用探针组合,同时采用2种方法进行细胞遗传学检测:实验组采用CD138免疫磁珠分选浆细胞后行荧光原位杂交技术(MACS-FISH)检测;对照组直接荧光原位杂交技术(D-FISH)检测。结果:30例MM患者,实验组采用CD138 MACS-FISH检出率为83.3%,对照组D-FISH法细胞遗传异常检出率为46.7%,两组差异具有统计学意义(p<0.05)。研究结果表明:分析不同类型的细胞遗传异常,MACS-FISH法1q21检出率为46.7%,RB1检出率为50.0%,Ig H检出率为70.0%,P53检出率为20.0%;D-FISH法检出率分别为23.3%,30.0%、36.7%、10.0%。通过细胞核型分析,30例MM患者中,发现5例患者为异常核型,仅为16.7%,其中1例患者为单一结构异常,复杂异常核型患者为4例。我们的研究结论表明:进行CD138免疫磁珠分选浆细胞的FISH技术在多发性骨髓瘤诊断应用中可显著提高细胞遗传学异常检测敏感性,具有临床推广应用的价值。     

Variation of wheatgrass chromosomes in wheat-wheatgrass alien addition line "TAI-27"revealed by fluorescence in situ hybridization (FISH)

Ｔｒａｎｓｆｅｒｏｆａｌｉｅｎｇｅｎｅｓｔｏｗｈｅａｔｔｈｒｏｕｇｈｃｈｒｏｍｏｓｏｍｅｅｎｇｉｎｅｅｒｉｎｇｉｓｏｎｅｏｆｔｈｅｉｍｐｏｒｔａｎｔｗａｙｓｔｏｉｍｐｒｏｖｅｗｈｅａｔｇｅｎｅｔｉｃｂａｃｋｇｒｏｕｎｄ.Ｔｈｅｂａｓｉｃｓｔｅｐｓｏｆｔｈｉｓｐｒｏｃｅｄｕｒｅａｒｅｆｉｒｓｔｔｏｔｒａｎｓｆｅｒａｌｉｅｎｃｈｒｏｍｏｓｏｍｅｓｉｎｔｏｗｈｅａｔ,ａｎｄｔｈｅｎｔｏｉｎｔｅｇｒａｔｅｔｈｅｕｓｅｆｕｌｇｅｎｅｓｏｆａｌｉｅｎｃｈｒｏｍｏｓｏｍｅｓｉｎｔｏｗｈｅａｔｃｈｒｏｍｏｓｏｍｅ…     

小麦异源易位系的高效诱导和分子细胞遗传学鉴定

利用杀配子染色体(gametocidal chromosome)和低剂量(10Gy)γ-射线辐射花粉两种方法诱导小麦(Triticum aestixum L)-滨麦(Leymus mollis Trin)和小麦-中间偃麦草[Thinopyrum intermedium(Host)Barkwarth]的易位系。通过基因组原位杂交(GISH)分析,在59个小滨麦代换系M8724-8-13与离果山羊草(Aegilops trincialis L)3C染色体附加系的杂交后代中获得了3株小麦-滨麦易位系,易位频率达到5．08％。其中1个易位系经C-分带证明是小麦的7D染色体与1条滨麦的染色体发生了整臂易位。同时还获得了3个滨麦染色体的缺失系。滨麦染色体发生结构变异的总频率为8．47％。除了滨麦染色体以外,在一些植株中还观察到小麦的染色体也发生了缺失。在69个普通小麦与小麦-中间偃麦草附加系TAI-14辐射花粉的杂交后代中,得到2株小麦-中间偃麦草的易位系,易位频率为2．90％。两个易位系都是小片段易位,经C-分带证明两个易位系所涉及的小麦染色体分别是3A和4A。利用杀配子染色体和低剂量γ射线辐射花粉诱导小麦异源易位系都是行之有效的方法,但这两种方法各有优缺点,在实际工作中应根据不同的目的选用不同的实验体系。     

免疫白粉病的小麦种内易位系的创制

以普通小麦Ａ５５２为父本、ＩＲＳ／ＩＢＬ黑麦和小麦易位系早抗为母本的杂种Ｓ３０６３,经Ｃ－分带和原位杂交鉴定,发现丢失了母本的黑麦成分,同时又发生了小麦种内易位,变成了５ＢＳ／７ＢＳ、５ＢＬ／７ＢＬ臂间双易位系。与此同时,白粉病抗性和一些农艺性状也发生了变化,此已己连续３年对白粉病免疫,且免疫条锈、叶锈和高抗黄矮病,每公顷５５２３千克,接近北京推广品种京冬６号     

荧光原位杂交技术在医学微生物学中的应用

以16S rRNA 为靶序列的寡核苷酸探针荧光原位杂交技术已广泛应用于分析复杂环境中的微生物群落构成,包括监测和鉴定病原微生物以及未被培养微生物．通过对临床样品中微生物细胞的检测能提供微生物在人体中的种类、数量和空间分布等信息．其结果快速准确,较之传统的病原微生物诊断方法具有明显的优越性,在临床应用中有广泛的前景．     

黄褐棉45S rDNA的FISH定位及核型分析

黄褐棉是棉属5个四倍体棉种之一,利用荧光原位杂交技术将45S rDNA定位在黄褐棉2、4、9号染色体,2号染色体上的45S rDNA特别大,信号位于随体并覆盖了染色体的短臂,比二倍体和四倍体棉种的45SrDNA都要大得多;另外的2对信号很小,形状与陆地棉中的弱信号类似。黄褐棉的核型公式为：2n=4x=52=50m（2SAT）＋2sm,属于2B类型,第2对染色体为亚中着丝粒染色体,其余都为中部着丝粒染色体。黄褐棉的核型、随体数、45S rDNA与其他四倍体棉种区别很大,黄褐棉是一个非常特殊的四倍体棉种。