Cross-reactivity in assays for prolactin and optimum screening policy for macroprolactinaemia

T. Smith, S. Kelly, M. Fahie-Wilson
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引用次数: 2

Abstract

Abstract Objectives Macroprolactin cross-reacts in immunoassays for prolactin causing apparent hyperprolactinaemia (macroprolactinaemia) and consequent misdiagnosis and mismanagement of patients. Methods We determined the prevalence of macroprolactinaemia using prolactin immunoassays with reported “high” (Tosoh) or “low” cross-reactivity (Roche) with macroprolactin. We additionally modelled the effects of increasing the screening threshold on workload and sensitivity in the detection of macroprolactinaemia. Results A review of routine requests for prolactin received in a 12 month period identified 670 sera with hyperprolactinaemia (Tosoh assay). Treatment with polyethylene glycol (PEG) precipitation demonstrated normal levels of monomeric prolactin in 165 sera (24.6%) indicating macroprolactinaemia. In the macroprolactinaemic cohort, total prolactin levels were lower with the Roche assay (473 ± 132 mU/L; mean ± SD) compared to the Tosoh assay (683 ± 217 mU/L), p < 0.005. The prevalence of macroprolactinaemia was also lower with the Roche assay (6.2%). The number of samples that required screening for macroprolactinaemia fell by 14% when Roche gender specific total prolactin reference limits were applied. Use of a higher screening threshold (700 mU/L) reduced the screening workload considerably (Roche by 45%, Tosoh by 37%) however, the sensitivity of detection of macroprolactinaemia decreased markedly (Roche 90%, Tosoh 59%). Conclusions Macroprolactin interferes in both Tosoh and Roche prolactin immunoassays. Use of an assay with a relatively low cross reactivity with macroprolactin, e.g. Roche, will lead to a modest reduction in the screening workload. Increasing the screening threshold above the upper limit of the assay reference interval will also reduce the screening workload but leads to disproportionate increases in the number of cases of macroprolactinaemia which are missed.
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催乳素检测的交叉反应性及大催乳素血症的最佳筛选策略
目的在催乳素免疫检测中,催乳素交叉反应引起明显的高催乳素血症(macroprolactinaemia),导致患者误诊和管理不当。方法:我们使用催乳素免疫测定法测定大催乳素血症的患病率,报告的催乳素与大催乳素的交叉反应性“高”(Tosoh)或“低”(Roche)。我们还模拟了增加筛查阈值对工作量和检测巨催乳素血症敏感性的影响。结果对12个月期间收到的常规催乳素要求进行审查,确定670份血清患有高催乳素血症(Tosoh测定)。聚乙二醇(PEG)沉淀治疗显示165份血清中单体催乳素水平正常(24.6%),提示大量催乳素血症。在巨催乳素血症队列中,罗氏测定总催乳素水平较低(473±132 mU/L;平均±SD),与Tosoh法(683±217 mU/L)相比,p < 0.005。罗氏测定的大泌乳素血症患病率也较低(6.2%)。当采用罗氏特定性别的总催乳素参考限量时,需要筛查大量催乳素血症的样本数量下降了14%。使用更高的筛选阈值(700 mU/L)大大减少了筛选工作量(罗氏减少45%,Tosoh减少37%),但检测巨泌乳素血症的敏感性明显下降(罗氏90%,Tosoh 59%)。结论巨催乳素对Tosoh和Roche催乳素免疫检测均有干扰作用。使用与大催乳素交叉反应性相对较低的检测方法,例如罗氏,将导致筛选工作量的适度减少。将筛查阈值提高到高于测定参考区间上限的水平,也将减少筛查工作量,但会导致漏诊的大量泌乳素血症病例数量不成比例地增加。
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