小腿晶状体左旋Z-DNA序列的固定和免疫定位。

Lens and eye toxicity research Pub Date : 1991-01-01
C E Gagna, O G Mitchell, J H Chen
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引用次数: 0

摘要

为了确定正常晶状体中是否存在Z-DNA序列并确定其结构-功能关系,采用免疫组织化学方法对固定和未固定的小牛晶状体组织切片进行检测。以溴化(Br-) poly(dG-dC).poly(dG-dC)为抗原,制备多克隆和单克隆抗z - dna抗体作为免疫探针。z -螺旋抗原的结构通过圆二色性(CD)和紫外光谱证实。全兔、山羊抗z - dna血清;兔、山羊IgG多克隆抗z - dna抗体;利用抗Z-DNA单克隆IgG抗体作为Z-DNA免疫探针,定位小牛晶状体组织切片中的Z-DNA。采用过氧化物酶-抗过氧化物酶(PAP)免疫组化检查,晶状体皮质区与抗z - dna抗体反应强烈,而晶状体核区未见免疫反应。全血清、亲和纯化IgG多克隆抗体和单克隆抗体均获得相似的免疫反应模式。在非固定晶状体组织切片中,抗z - dna抗体的免疫结合较低,为有效的背景型结合。我们测试了各种固定剂,以探索小牛晶状体组织中潜在的抗体- z - dna相互作用。核固定剂增强Z-DNA抗体的免疫反应性,而福尔马林、微解剖和细胞质固定剂产生的效果较小。用DNase I消化晶状体组织可以消除Z-DNA的免疫反应性,而RNase A和RNase T1处理则没有效果。放线菌素D也能抑制Z-DNA的免疫反应性。
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Fixation and immunolocalization of left-handed Z-DNA sequences in the calf lens.

In order to establish the presence of Z-DNA sequences in the normal crystalline lens and to define their structure-function relationship, fixed and unfixed calf lens tissue sections were examined immunohistochemically. Polyclonal and monoclonal anti-Z-DNA antibodies were developed as immunoprobes, using brominated (Br-) poly(dG-dC).poly(dG-dC) as an antigen. The structure of the Z-helix antigen was confirmed by circular dichroism (CD) and U.V. spectroscopy. Whole rabbit and goat anti-Z-DNA sera; rabbit and goat IgG polyclonal anti-Z-DNA antibodies; and anti-Z-DNA monoclonal IgG antibodies were utilized as Z-DNA immunoprobes to localize the Z-DNA in calf lens tissue sections. Immunohistochemical examination using the peroxidase-antiperoxidase (PAP) method indicated that the cortex region of the lens reacted strongly with the anti-Z-DNA antibodies, while no immunoreaction could be observed in the nucleus region. Similar immunoreactive patterns were obtained whether whole sera, affinity purified IgG polyclonal antibodies or monoclonal antibodies were utilized. Immunobinding of anti-Z-DNA antibodies was low, effectively background type binding, in unfixed lens tissue sections. Various fixatives were tested to explore the potential antibody-Z-DNA interaction in calf lens tissue. Nuclear fixatives enhanced Z-DNA antibody immunoreactivity, while formalin, microanatomic and cytoplasmic fixatives produced lesser results. Digestion of the lens tissue with DNase I eliminated Z-DNA immunoreactivity, while RNase A and RNase T1 treatment had no effect. Actinomycin D also prevented Z-DNA immunoreactivity.

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