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培养的交感神经元神经突延伸的模式和动力学与年龄有关。

Patterns and kinetics of neurite extension from sympathetic neurons in culture are age dependent.

作者信息

Argiro V, Johnson M I

出版信息

J Neurosci. 1982 Apr;2(4):503-12. doi: 10.1523/JNEUROSCI.02-04-00503.1982.

Abstract

Long term (2- to 3-week) cultures of superior cervical ganglia (SCG) were established from rats and rat embryos ranging in age from 15 days of gestation (E15) to 279 days postnatal (P279). Cultures were grown on a collagen substratum and fed a serum-containing medium with added nerve growth factor. Radial outgrowth of neurites was measured as a function of time for up to 2 to 3 weeks. Computer-aided analysis generated estimates of onset time, initial rate, and subsequent changes in the rate of growth of these neurites. The explants from perinatal rats showed the fastest growth onset time (5 to 13 hr), fastest initial rate of growth (370 to 660 microns/d), and a decline in growth rate during the first 2 weeks in culture. The outgrowth from these perinatal explants was composed of many small fascicles. Neurites from the prenatal explants (E15 to E20) began to grow within 22 hr in vitro. Their rate of growth was lower initially (150 to 300 microns/d) but increased to equal the perinatal explant initial rate before again falling to an intermediate level (200 to 300 microns/d). The outgrowth from prenatal explants contained fewer larger fascicles. Postnatal explants had low initial rates of growth (70 to 176 microns/d) but exhibited an increasing growth rate in vitro, again approaching an intermediate rate of 200 to 250 microns/d after 2 to 3 weeks. Neurite outgrowth from the postnatal explants was delayed by an amount roughly correlated with the age of the animal advancing postnatal age but reached an asymptote of about 50 to 150 microns/d at about P30. The outgrowth was initially sparse but became denser with time in culture. Thus, in a culture system in which medium composition and growth substratum are held constant, marked differences can be observed in pattern, latency, initial rate, and subsequent changes in rate of neurite extension among SCG explants from different ages of rats and rat embryos.

摘要

从妊娠15天(E15)至出生后279天(P279)的大鼠和大鼠胚胎中建立颈上神经节(SCG)的长期(2至3周)培养物。培养物在胶原蛋白基质上生长,并喂食添加了神经生长因子的含血清培养基。测量神经突的放射状生长长达2至3周的时间函数。计算机辅助分析生成了这些神经突生长的起始时间、初始速率和后续速率变化的估计值。围产期大鼠的外植体显示出最快的生长起始时间(5至13小时)、最快的初始生长速率(370至660微米/天),并且在培养的前2周内生长速率下降。这些围产期外植体的生长由许多小束组成。产前外植体(E15至E20)的神经突在体外22小时内开始生长。它们的生长速率最初较低(150至300微米/天),但在再次降至中间水平(200至300微米/天)之前增加到与围产期外植体的初始速率相等。产前外植体的生长包含较少的较大束。产后外植体的初始生长速率较低(70至176微米/天),但在体外表现出增加的生长速率,在2至3周后再次接近200至250微米/天的中间速率。产后外植体的神经突生长延迟的量大致与动物出生后年龄的增加相关,但在约P30时达到约50至150微米/天的渐近线。生长最初稀疏,但随着培养时间的推移变得更密集。因此,在培养基组成和生长基质保持恒定的培养系统中,可以观察到来自不同年龄大鼠和大鼠胚胎的SCG外植体在神经突延伸的模式、潜伏期、初始速率和后续速率变化方面存在明显差异。

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