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首页> 外文期刊>Journal of neurotrauma >Detection of single- and double-strand DNA breaks after traumatic brain injury in rats: comparison of in situ labeling techniques using DNA polymerase I, the Klenow fragment of DNA polymerase I, and terminal deoxynucleotidyl transferase.
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Detection of single- and double-strand DNA breaks after traumatic brain injury in rats: comparison of in situ labeling techniques using DNA polymerase I, the Klenow fragment of DNA polymerase I, and terminal deoxynucleotidyl transferase.

机译:大鼠脑外伤后单链和双链DNA断裂的检测:使用DNA聚合酶I,DNA聚合酶I的Klenow片段和末端脱氧核苷酸转移酶的原位标记技术的比较。

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摘要

DNA damage is a common sequela of traumatic brain injury (TBI). Available techniques for the in situ identification of DNA damage include DNA polymerase I-mediated biotin-dATP nick-translation (PANT), the Klenow fragment of DNA polymerase I-mediated biotin-dATP nick-end labeling (Klenow), and terminal deoxynucleotidyl transferase-mediated dUTP nick-end labeling (TUNEL). While TUNEL has been widely utilized to detect primarily double-strand DNA breaks, the use of PANT to detect primarily single-strand DNA breaks and Klenow to detect both single- and double-strand DNA breaks has not been reported after TBI. Accordingly, coronal brain sections from naive rats and rats at 0, 0.5, 1, 2, 6, 24, and 72 h (n = 3-5/group) after controlled cortical impact with imposed secondary insult were processed using the PANT, Klenow, and TUNEL methods. Cells with DNA breaks were detected by PANT in the ipsilateral hemisphere as early as 0.5 h after injury and were maximal at 6 h (cortex = 66.3+/-15.8, dentate gyrus 58.6+/-12.8, CA1 = 15.8+/-5.9, CA3 = 12.8+/-4.2 cells/x 400 field, mean +/- SEM, all p < 0.05 versus naive). Cells with DNA breaks were detected by Klenow as early as 30 min and were maximal at 24 h (cortex = 56.3+/-14.3, dentate gyrus 78.0+/-16.7, CA1 = 25.8+/-4.7, CA3 = 29.3+/-15.1 cells/x 400 field, all p < 0.05 versus naive). Cells with DNA breaks were not detected by TUNEL until 2 h and were maximal at 24 h (cortex = 47.7+/-21.4, dentate gyrus 63.0+/-11.9, CA1 = 5.6+/-5.4, CA3 = 6.9+/-3.7 cells/x 400 field, cortex and dentate gyrus p < 0.05 versus naive). Dual-label immunofluorescence revealed that PANT-positive cells were predominately neurons. These data demonstrate that TBI results in extensive DNA damage, which includes both single- and double-strand breaks in injured cortex and hippocampus. The presence of multiple types of DNA breaks implicate several pathways in the evolution of DNA damage after TBI.
机译:DNA损伤是颅脑外伤(TBI)的常见后遗症。用于DNA损伤原位鉴定的可用技术包括DNA聚合酶I介导的生物素-dATP缺口翻译(PANT),DNA聚合酶I介导的生物素-dATP缺口末端标记的Klenow片段(Klenow)和末端脱氧核苷酸转移酶介导的dUTP缺口末端标记(TUNEL)。虽然TUNEL已被广泛用于检测主要的双链DNA断裂,但是在TBI之后尚未见到使用PANT来检测主要的单链DNA断裂和使用Klenow来检测单链和双链DNA断裂。因此,使用PANT,Klenow处理了在受到皮层控制并施加了二次侮辱之后,在0、0.5、1、2、6、24和72小时(n = 3-5 /组)从幼稚大鼠和大鼠的冠状脑切片和TUNEL方法。最早在受伤后0.5小时通过PANT在同侧半球中检测到具有DNA断裂的细胞,并且在6小时时达到最大值(皮质= 66.3 +/- 15.8,齿状回58.6 +/- 12.8,CA1 = 15.8 +/- 5.9, CA3 = 12.8 +/- 4.2细胞/ x 400视野,平均值+/- SEM,相对于天真,所有p <0.05。 Klenow最早在30分钟时检测到具有DNA断裂的细胞,并在24 h时最大(皮质= 56.3 +/- 14.3,齿状回78.0 +/- 16.7,CA1 = 25.8 +/- 4.7,CA3 = 29.3 +/- 15.1个像元/ x 400视场,相对于天真而言,所有p <0.05。 TUNEL直到2 h才检测到具有DNA断裂的细胞,并且在24 h时最大(皮质= 47.7 +/- 21.4,齿状回63.0 +/- 11.9,CA1 = 5.6 +/- 5.4,CA3 = 6.9 +/- 3.7细胞/ x 400视野,皮层和齿状回p(相对于天真而言,p <0.05)。双标记免疫荧光显示PANT阳性细胞主要是神经元。这些数据表明,TBI导致广泛的DNA损伤,包括受损皮层和海马的单链和双链断裂。 TBI后,DNA断裂的多种类型暗示了DNA损伤演变的几种途径。

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