吸收期对生长大鼠肌肉和肝脏蛋白质合成率的影响。

S Dänicke, R Nieto, G E Lobley, M F Fuller, D S Brown, E Milne, A G Calder, S Chen, I Grant, W Böttcher
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引用次数: 10

摘要

在生长中的雄性大鼠中,使用大剂量技术,在暴露于[15N]苯丙氨酸10分钟的基础上,测试了进餐后时间(30,60,90和120分钟)对肝脏和腓肠肌蛋白质合成的影响。分数合成率由组织蛋白结合苯丙氨酸和游离标记苯丙氨酸的原子百分数之间的比率估计。后者采用叔丁基二甲基硅基氨基酸衍生物气相色谱质谱法测定。利用氨基酸制备层析法将腓肠肌蛋白结合苯丙氨酸与其他氨基酸分离,然后在连接连续流同位素比质谱仪(IRMS)的自动碳氮Roboprep (CN)燃烧模块中氧化成N2,监测m/z离子28和29。用附在样品制备模块上的气相色谱仪和同位素比质谱仪(GC - irms)分离肝脏中的蛋白结合苯丙氨酸,再次监测28和29的m/z离子。结果表明:145 g大鼠禁食12 h后,腓肠肌和肝脏的每日蛋白质合成率分别为13.9%和65.6%。在摄食后30分钟内,肌肉和肝脏的ks分别增加到14.9%和91.8%,并在接下来的90分钟内保持在这些值(开始摄食后60分钟为14.6%和87.4%,开始摄食后120分钟为14.3%和88.6%)。结论是,吸收期蛋白质合成速率特征的测量可以在开始用餐后30分钟至2小时内进行,而ks值没有显着变化。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Responses in the absorptive phase in muscle and liver protein synthesis rates of growing rats.

The effect of time after beginning of a meal (30, 60, 90 and 120 min) on liver and gastrocnemius muscle protein synthesis was tested in growing male rats using the large dose technique, based on a 10 min exposure to [15N]phenylalanine. The fractional synthesis rate was estimated from the ratio between the atom percent excess of tissue protein-bound and free labelled phenylalanine. The latter was measured by gas chromatography mass spectrometry using the tertiary-butyldimethylsilyl amino acid derivatives. The protein-bound phenylalanine of gastrocnemius muscle was separated from the other amino acids using preparative amino acid chromatography and then oxidised to N2 in an automated carbon-nitrogen Roboprep (CN) combustion module attached to a continuous flow isotope ratio mass spectrometer (IRMS), with m/z ions 28 and 29 monitored. The protein-bound phenylalanine from liver was separated by a gas chromatograph attached to a sample preparation module and an isotope ratio mass spectrometer (GC C-IRMS), with again m/z ions of 28 and 29 monitored. The following results were obtained: the daily fractional protein synthesis rates (ks) in gastrocnemius muscle and liver were 13.9% and 65.6% respectively, in 12 h fasted 145 g rats. These ks increased within 30 min after ingestion of meal to 14.9% and 91.8% for muscle and liver, respectively, and remained at these values for the next 90 min (14.6% and 87.4% at 60 min, and 14.3% and 88.6% at 120 min after the beginning of feeding). It was concluded that measurement of protein synthesis rates characteristics for the absorptive phase can be undertaken in a period from thirty minutes to two hours after start of a meal, without significant changes in the ks values.

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