分析试验室
分析試驗室
분석시험실
ANALYTICAL LABORATORY
2009年
12期
9-13
,共5页
崔凤灵%闫迎华%张强斋%渠桂荣%卢雁
崔鳳靈%閆迎華%張彊齋%渠桂榮%盧雁
최봉령%염영화%장강재%거계영%로안
脱氧尿苷%人血清白蛋白(HSA)%考马斯亮蓝G250(CBB)%同步荧光光谱%分子探针
脫氧尿苷%人血清白蛋白(HSA)%攷馬斯亮藍G250(CBB)%同步熒光光譜%分子探針
탈양뇨감%인혈청백단백(HSA)%고마사량람G250(CBB)%동보형광광보%분자탐침
2'-Deoxyuridine%Human serum albumin%Coomassie brilliant blue G-250%Synchronous fluorescence spectra%Molecular probe
最佳实验条件下,基于脱氧尿苷与人血清白蛋白(HSA)相互作用,导致血清白蛋白的同步荧光光谱发生特异性变化,且体系的同步荧光强度和溶液中白蛋白的浓度呈良好的线性关系,建立了以脱氧尿苷为探针,运用固定波长同步荧光光谱快速测定生物样品中蛋白质总含量的新方法.深入考察了△λ值、反应介质、试剂用量、离子强度、加入顺序、反应时间等因素对测定的影响.在最佳实验条件下,体系的同步荧光强度与血清白蛋白在2.76~524.4μg/mL范围内的线性相关系数为0.9991,方法的检出限可达0.11μg/mL.运用本方法对人血清、唾液和尿液等生物样品进行测定并进行加标回收实验,回收率在98.0%~102.5%之间.对11份空白溶液进行平行测定,相对标准差为1.2%.用经典的考马斯亮蓝G-250(CBB)法做了对照实验,两种方法测定结果基本一致.还考察了一些常见离子和有机物存在时对蛋白质测定的影响.本方法已用于血清、唾液和尿样等生物样品中蛋白质总量的快速测定.
最佳實驗條件下,基于脫氧尿苷與人血清白蛋白(HSA)相互作用,導緻血清白蛋白的同步熒光光譜髮生特異性變化,且體繫的同步熒光彊度和溶液中白蛋白的濃度呈良好的線性關繫,建立瞭以脫氧尿苷為探針,運用固定波長同步熒光光譜快速測定生物樣品中蛋白質總含量的新方法.深入攷察瞭△λ值、反應介質、試劑用量、離子彊度、加入順序、反應時間等因素對測定的影響.在最佳實驗條件下,體繫的同步熒光彊度與血清白蛋白在2.76~524.4μg/mL範圍內的線性相關繫數為0.9991,方法的檢齣限可達0.11μg/mL.運用本方法對人血清、唾液和尿液等生物樣品進行測定併進行加標迴收實驗,迴收率在98.0%~102.5%之間.對11份空白溶液進行平行測定,相對標準差為1.2%.用經典的攷馬斯亮藍G-250(CBB)法做瞭對照實驗,兩種方法測定結果基本一緻.還攷察瞭一些常見離子和有機物存在時對蛋白質測定的影響.本方法已用于血清、唾液和尿樣等生物樣品中蛋白質總量的快速測定.
최가실험조건하,기우탈양뇨감여인혈청백단백(HSA)상호작용,도치혈청백단백적동보형광광보발생특이성변화,차체계적동보형광강도화용액중백단백적농도정량호적선성관계,건립료이탈양뇨감위탐침,운용고정파장동보형광광보쾌속측정생물양품중단백질총함량적신방법.심입고찰료△λ치、반응개질、시제용량、리자강도、가입순서、반응시간등인소대측정적영향.재최가실험조건하,체계적동보형광강도여혈청백단백재2.76~524.4μg/mL범위내적선성상관계수위0.9991,방법적검출한가체0.11μg/mL.운용본방법대인혈청、타액화뇨액등생물양품진행측정병진행가표회수실험,회수솔재98.0%~102.5%지간.대11빈공백용액진행평행측정,상대표준차위1.2%.용경전적고마사량람G-250(CBB)법주료대조실험,량충방법측정결과기본일치.환고찰료일사상견리자화유궤물존재시대단백질측정적영향.본방법이용우혈청、타액화뇨양등생물양품중단백질총량적쾌속측정.
Under the optimum experimental conditions, 2'-Deoxyuridine could interact with human serum albumin (HSA), resulting in the specific changes of the intrinsic fluorescence of serum albumin. Synchronous fluorescence in-tensity of the system had a good linear relationship with the serum albumin concentration in the range of 2.76~524.4 μg/mL, and the detection limit of this method was 0.11 μg/mL. A novel method for the determination of the proteins with 2'-Deoxyufidine as a molecular probe was developed. The effect factors for spectral characterization and intensity of synchronous fluorescence such as the value of △λ, reaction medium, reagent concentration, ionic strength, addition sequence, reaction time were also investigated. The recoveries were 98.0%~102.5% and 11 blank solut-ions to the parallel experimental data obtained the relative standard deviation of 1.12%. The CBB G-250 method was done as the control experiment and the results were in good accordance with those by synchronous fluorescence method. The results indicated that this method was simple, rapid, and had high sensitivity, wide linear range, good stability and high selectivity. It was successfully applied to the determination of the total proteins in human body fluids such as human serum, saliva and urine samples, and the results were satisfactory.
