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死后间隔时间对DNA寡核小体原位末端标记的影响。

Effect of postmortem interval on in situ end-labeling of DNA oligonucleosomes.

作者信息

Petito C K, Roberts B

机构信息

Department of Pathology (Neuropathology), University of Miami School of Medicine, Florida, USA.

出版信息

J Neuropathol Exp Neurol. 1995 Nov;54(6):761-5. doi: 10.1097/00005072-199511000-00002.

Abstract

In situ end-labeling (ISEL) of DNA oligonucleosomes facilitates detection of apoptosis in tissue sections by binding labeled nucleotides to the oligonucleosomal fragments. Although ISEL is used in postmortem material, the effect of autolysis is not specifically known. Accordingly, normal rat brain and intestine were immersed in formalin after postmortem intervals (PMI) from 0 to 72 hours (h) or were fixed by perfusion with ethanol or paraformaldehyde-glutaraldehyde (PF-G). Omission of the binding enzymes or pretreatment with DNAase served as negative and positive controls. With DNA polymerase, material fixed by perfusion or by formalin immersion with PMI of O contained ISEL-positive nuclei only in apical intestinal cells and rare intravascular blood cells in brain. Postmortem intervals from 8 to 72 h did not alter this staining pattern although false-positive ISEL developed at section edges as a result of tissue drying. Terminal deoxynucleotidyl transferase gave similar results in the formalin-fixed material with PMI from 0-48 h but nonspecific nuclear labeling was increased with a PMI of 72 h and was widespread in the PF-G and ethanol-perfused material. This study shows that PMI of at least 72 h do not affect the sensitivity or the specificity of ISEL and confirm the reliability of this procedure in postmortem material. The results also indicate that false-positive ISEL occurs if the tissue is allowed to dry or if certain combinations of fixatives and binding enzymes are used.

摘要

DNA寡核小体的原位末端标记(ISEL)通过将标记的核苷酸与寡核小体片段结合,便于在组织切片中检测细胞凋亡。尽管ISEL用于尸检材料,但自溶的影响尚不清楚。因此,将正常大鼠的脑和肠在死后间隔时间(PMI)从0至72小时(h)后浸入福尔马林中,或通过用乙醇或多聚甲醛-戊二醛(PF-G)灌注进行固定。省略结合酶或用DNA酶预处理作为阴性和阳性对照。使用DNA聚合酶时,PMI为0时通过灌注或福尔马林浸泡固定的材料仅在肠顶端细胞中含有ISEL阳性核,在脑中仅有罕见的血管内血细胞含有ISEL阳性核。尽管由于组织干燥在切片边缘出现了假阳性ISEL,但死后间隔时间从8至72小时并未改变这种染色模式。末端脱氧核苷酸转移酶在PMI为0至48小时的福尔马林固定材料中得到了类似的结果,但PMI为72小时时非特异性核标记增加,并且在PF-G和乙醇灌注的材料中广泛存在。本研究表明,至少72小时的PMI不会影响ISEL的敏感性或特异性,并证实了该方法在尸检材料中的可靠性。结果还表明,如果组织干燥或使用某些固定剂和结合酶的组合,会出现假阳性ISEL。

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