尿试纸与微量白蛋白尿定量方法的比较。

M J Pugia, J A Lott, L W Clark, D R Parker, J F Wallace, T W Willis
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引用次数: 0

摘要

我们描述了一种新的浸读量尺,可以检测尿白蛋白浓度为10mg /l及以上,尿肌酐浓度为300mg /l及以上。白蛋白检测基于高亲和力染料结合技术,而肌酐检测基于铜肌酐复合物的过氧化物酶样活性。使用这两种测试试纸,从正常成年人补充白蛋白和肌酐的尿液被正确地识别为两种分析物的期望值的+/- 15%以内;日间变异系数为7.1% ~ 16.1%。我们用拜耳和勃林格曼海姆微量检测白蛋白试纸对275例患者的未修改尿液进行了检测,并用贝克曼阵列对相同样本进行了白蛋白检测。我们还用另一种定量免疫化学方法和电泳加总蛋白法分析了275组中42例尿液的白蛋白浓度。定量免疫化学方法似乎低估了尿白蛋白浓度;在这42例尿液中,通过一种定量方法检测为阴性,即<约16-20 mg/l,但通过拜耳试纸检测为阳性,其中电泳/总蛋白测定联合检测为阳性的有33例。拜耳白蛋白试纸正确鉴别尿液< 16mg /l或>或= 16mg /l的比率为80%。当浓度为20 mg/l时,转化率提高到87%。我们还使用拜耳双垫试纸测定了275例患者的尿白蛋白/肌酐比率,发现84%的时间与定量免疫化学法测定白蛋白和率-贾菲法测定肌酐的相同比率一致;以30的白蛋白/肌酐比值(mg/g)作为鉴别点。在贝克曼阵列患者的6个新鲜尿液中进行的白蛋白稳定性研究显示,在-20℃储存一个月后,白蛋白稳定性下降幅度小但持续下降,而在4℃储存一个月后则没有下降。在这些储存条件下,通过电泳/总蛋白和试纸来估计的人造尿中的白蛋白没有变化。1 g/l的硼酸作为尿液防腐剂,对用本文所述的任何方法测量白蛋白和测定肌酐都没有影响。在异常排泄率下存在的其他尿蛋白不干扰拜耳白蛋白试纸。尿中胆红素、柠檬酸、肌酸、抗坏血酸、白蛋白、血红蛋白和肌红蛋白的异常浓度不影响肌酸酐试纸的测量。上述前四项不影响拜耳试纸检测白蛋白的结果。
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Comparison of urine dipsticks with quantitative methods for microalbuminuria.

We describe a new dip- and read dipstick that detects urine albumin at concentrations of 10 mg/l and above and urine creatinine at concentrations of 300 mg/l and above. The albumin assay is based on a high-affinity, dye-binding technique while the creatinine assay is based on the peroxidase-like activity of copper creatinine complexes. With these two-test dipsticks, urines from normal adults supplemented with albumin and creatinine were correctly identified to within +/- 15% of the expected value for both analytes; the between-day coefficients of variation ranged from 7.1% to 16.1%. We tested 275 patients' unmodified urines by the Bayer and Boehringer Mannheim Micral-Test albumin dipsticks and for albumin with the Beckman Array on the same specimens. We also analyzed 42 selected urines from the group of 275 for albumin by another quantitative immunochemical method and by electrophoresis plus a total protein method to estimate the albumin concentration. The quantitative immunochemical methods appear to underestimate the urine albumin concentrations; in these 42 urines measured as negative, i.e., < ca. 16-20 mg/l, by one of the quantitative method but positive by the Bayer dipstick, 33 of these were positive by the electrophoresis/total protein assay combination. The Bayer albumin dipstick correctly identified urines as having < 16 mg/l or > or = 16 mg/l at an 80% rate. At a cutoff of 20 mg/l, the rate increased to 87%. We also determined the urinary albumin/creatinine ratios on the 275 patients using the Bayer two-pad dipstick and found agreement 84% of the time with the same ratio obtained from a quantitative immunochemical method for albumin and a rate-Jaffe method for creatinine; an albumin/creatinine ratio (mg/g) of 30 was used as the discrimination point. Albumin stability studies performed on the Beckman Array patients with six fresh urines showed small but consistent decreases at -20 degrees C but not at 4 degrees C after one month of storage. The albumin in contrived urines, as estimated by electrophoreses/total protein and by the dipsticks did not change at these storage conditions. Boric acid at 1 g/l as a urine preservative had no effect on the measurement of albumin by any of the methods described here nor of the assay of creatinine. Other urinary proteins present at abnormal excretion rates did not interfere with the Bayer albumin dipstick. Abnormal concentrations of bilirubin, citrate, creatine, ascorbic acid, albumin, hemoglobin and myoglobin in urine did not interfere with the creatinine dipstick measurements. The first four of the above did not affect the Bayer dipstick results for albumin.

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