人体静脉血和毛细血管血中血清 25 羟维生素 D 水平的两种检测方法之间的相关性和一致性

Yutong Xing, Kaixi Wang, Xinyu Ma, Huifeng Zhang, Xiaoyu Tian
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引用次数: 0

摘要

该研究评估了 42 名健康成年人在补充维生素 D3 后同时采集的毛细血管和静脉血浆中 25- 羟维生素 D [25(OH)D] 水平的相关性和一致性。采用随机数字表法将他们随机分为三组。A 组每天服用 1,000 IU 维生素 D3,B 组每 10 天服用 10,000 IU 维生素 D3,C 组每 30 天服用 30,000 IU 维生素 D3,直到第 12 个月结束。分别在第 1 天、第 14 天、第 28 天、第 6 个月和第 12 个月用化学发光免疫分析法(CLIA)和质谱法(LC-MS)检测静脉血血清 25(OH)D 水平,同时用化学发光免疫分析法(CLIA)检测毛细血管血血清 25(OH)D 水平。采用皮尔逊相关分析和线性回归分析来研究两个样本的检测结果与同一样本中不同检测方法所得结果之间的关系和转换方程。Bland-Altman法、Kappa分析和接收者操作特征曲线(ROC)用于评估一致性、灵敏度和特异性。A 组的平均水平高于 B 组和 C 组(P < 0.001)。用 LC-MS 和 CLIA 测得的 42 名健康成人血清中 25(OH)D 的平均值分别为 45.32 nmol/L 和 49.88 nmol/L,用 LC-MS 测得的毛细血管血中 25(OH)D 的平均值为 52.03 nmol/L,差异有统计学意义(P < 0.001)。皮尔逊相关分析表明,散点数据的线性拟合公式为:静脉血 25(OH)D 浓度(nmol/L)= 1.105 * 毛细血管 25(OH)D 浓度 -7.532 nmol/L,R2 = 0.625。在临床诊断中,静脉和校正毛细血管 25(OH)D 水平之间的一致性很好(Kappa 值为 0.75)。毛细管血中调整后的血清 25(OH)D 具有较高的临床预测价值。当测量的 25(OH)D 水平较高时,两种方法的一致性较好。标准化的毛细管血化学发光法可用于 25(OH)D 的检测。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Correlation and consistency between two detection methods for serum 25 hydroxyvitamin D levels in human venous blood and capillary blood
The study assessed the correlation and concordance of 25-hydroxyvitamin D [25(OH)D] levels in capillary and venous plasma collected simultaneously after vitamin D3 supplementation in 42 healthy adults. They were randomly divided into three groups by random number table method. Group A took 1,000 IU vitamin D3 daily, group B took 10,000 IU vitamin D3 every 10 days, and group C took 30,000 IU vitamin D3 every 30 days until the end of the 12th month. Venous blood serum 25(OH)D level was detected by chemiluminescence immunoassay (CLIA) and mass spectrometry (LC-MS) at day 1, day 14, day 28, month 6, and month 12 respectively, the capillary blood serum 25(OH)D level was detected by chemiluminescence immunoassay (CLIA) at the same time. Pearson correlation analysis and linear regression analysis were employed to investigate the relationship and transformation equation between the findings of the two samples and the results obtained from different detection methods within the same sample. The Bland-Altman method, Kappa analysis, and receiver operating characteristic (ROC) curve were utilized for assessing consistency, sensitivity, and specificity.The three groups all reached a stable peak at 6 months, and the average levels of the three groups were 49.21, 42.50 and 43.025 nmol/L, respectively. The average levels of group A were higher than those of group B and group C (P < 0.001). The mean values of serum 25(OH)D measured by LC-MS and CLIA in 42 healthy adults were 45.32 nmol/L and 49.88 nmol/L, respectively, and the mean values of 25(OH)D measured by LC-MS in capillary blood were 52.03 nmol/L, and the difference was statistically significant (P < 0.001). Pearson correlation analysis showed that the linear fitting formula of scatter data was as follows: venous 25(OH)D concentration (nmol/L) = 1.105 * capillary 25(OH)D concentration −7.532 nmol/L, R2 = 0.625. Good agreement was observed between venous and corrected capillary 25(OH)D levels in clinical diagnosis (Kappa value 0.75). The adjusted serum 25(OH)D in capillary blood had a high clinical predictive value.The agreement between the two methods is good when the measured 25(OH)D level is higher. Standardized capillary blood chemiluminescence method can be used for 25(OH)D detection.
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