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损伤后大鼠磨牙去神经支配诱导的细胞增殖变化。

Denervation-induced changes in cell proliferation in the rat molar after wounding.

作者信息

Chiego D J, Klein R M, Avery J K, Gruhl I M

出版信息

Anat Rec. 1986 Apr;214(4):348-52. doi: 10.1002/ar.1092140403.

Abstract

The dental pulp has the capacity to initiate and maintain repair after trauma. The purpose of the present study was to quantitatively analyze the role of the peripheral nervous system in regulation of pulpal cell proliferation in response to wounding. Six groups of ten rats were used in these studies. There was one baseline group (wounded, but innervation intact) and five resection groups. The resection groups included rats with unilateral superior cervical ganglionectomy (SCG), unilateral inferior alveolar nerve resection (IAN), unilateral chorda tympani (CT) resection, IAN + SCG, or a complete unilateral nerve resection (IAN + SCG + CT). One millimeter of enamel and dentin was removed from the first mandibular molar on the experimental (resected) side. Therefore, each rat had an experimental and control molar. Rats were killed at various intervals from day 0 to day 15 after wounding and received 0.5 muCi/g b.wt. 3H-thymidine 1 hour before death. For the baseline (innervation intact) data a peak in 3H-thymidine incorporation occurred at 5 days after wounding. In the resected groups, there was a general increase in the number of labeled cells at the zero time point, and a suppression of the 5-day peak with a delay in the proliferative response to wounding. The SCG + IAN-resected group maintained the lowest number of labeled cells throughout the entire experimental period compared to the experimental baseline data and the two controls. At the initial and termination points the SCG + IAN-resected groups demonstrated the highest number of labeled cells.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

牙髓具有在创伤后启动并维持修复的能力。本研究的目的是定量分析外周神经系统在调节牙髓细胞对创伤的增殖反应中的作用。这些研究使用了六组,每组十只大鼠。有一个基线组(受伤但神经支配完整)和五个切除组。切除组包括单侧颈上神经节切除术(SCG)、单侧下牙槽神经切除术(IAN)、单侧鼓索神经(CT)切除术、IAN + SCG或完全单侧神经切除术(IAN + SCG + CT)的大鼠。从实验(切除)侧的第一下颌磨牙去除一毫米的釉质和牙本质。因此,每只大鼠都有一颗实验磨牙和一颗对照磨牙。在受伤后的第0天至第15天的不同时间点处死大鼠,并在死亡前1小时给予0.5μCi/g体重的3H-胸腺嘧啶核苷。对于基线(神经支配完整)数据,3H-胸腺嘧啶核苷掺入在受伤后第5天出现峰值。在切除组中,零时间点标记细胞数量普遍增加,5天峰值受到抑制,对创伤的增殖反应延迟。与实验基线数据和两个对照组相比,SCG + IAN切除组在整个实验期间标记细胞数量保持最低。在初始和终点时,SCG + IAN切除组显示标记细胞数量最多。(摘要截断于250字)

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