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Atomic force microscopy of DNA-colloidal gold and DNA-protein complexes

机译:DNA胶体金和DNA蛋白质复合物的原子力显微镜

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Abstract: developing methods for random and site-specific labeling of individual DNA molecules to facilitate manipulation of fragments excised in the atomic force microscope (AFM) and for localization of specific DNA domains, such as protein binding sites and origins of replication. One successful method was to incorporate biotinylated nucleotides at random internal locations or specifically at the ends of linearized DNA molecules in vitro. Following complex formation with 5 nm diameter streptavidin-gold conjugates, chromatographic purification and passive adsorption of the complexes of mica, the biotinylated domains were easily localized in the AFM by virtue of the distinctive size and shape of the streptavidin-gold complex. In many cases unconjugated streptavidin (i.e., lacking gold) was also observed attached to the biotinylated DNA. A second approach to site-specific labeling of DNA for imaging in the AFM was to react DNA with restriction enzymes having sequence-specific binding properties. Like the unconjugated streptavidin-DNA complexes, these enzyme-DNA complexes were visible without attached colloidal gold. Efforts to image DNA labeled in vivo using bromodeoxyuridine (BrdU) and anti-BrdU antibodies are ongoing.!16
机译:摘要:开发了对单个DNA分子进行随机和位点特异性标记的方法,以促进在原子力显微镜(AFM)中切除的片段的操纵以及对特定DNA域的定位,例如蛋白质结合位点和复制起点。一种成功的方法是在体外在随机内部位置或特别是在线性化DNA分子的末端掺入生物素化核苷酸。用直径5 nm的链霉亲和素-金结合物形成复合物,色谱纯化和云母复合物的被动吸附后,由于链霉亲和素-金复合物的独特大小和形状,生物素化结构域很容易位于AFM中。在许多情况下,还观察到未缀合的抗生蛋白链菌素(即,缺乏金)附着于生物素化的DNA。用于在AFM中成像的DNA的位点特异性标记的第二种方法是使DNA与具有序列特异性结合特性的限制酶反应。像未结合的链霉亲和素-DNA复合物一样,这些酶-DNA复合物可见,没有附着的胶体金。正在努力使用溴脱氧尿苷(BrdU)和抗BrdU抗体对体内标记的DNA进行成像!16

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