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基于 HRP2 和 pLDH 的快速诊断检测在南苏丹阿韦尔疟疾评估及 pfhrp2/3 缺失情况。

Evaluation of HRP2 and pLDH-based rapid diagnostic tests for malaria and prevalence of pfhrp2/3 deletions in Aweil, South Sudan.

机构信息

Epicentre, 14-34 Avenue Jean Jaurès, Paris, France.

Médecins Sans Frontières, 14-34 Avenue Jean Jaurès, Paris, France.

出版信息

Malar J. 2022 Sep 9;21(1):261. doi: 10.1186/s12936-022-04280-w.

Abstract

BACKGROUND

Rapid diagnostic tests (RDT) for malaria are the primary tool for malaria diagnosis in sub-Saharan Africa but the utility of the most commonly used histidine-rich protein 2 (HRP2) antigen-based tests is limited in high transmission settings due to the long duration of positivity after successful malaria treatment. HRP2 tests are also threatened by the emergence of Plasmodium that do not carry pfhrp2 or pfhrp 3 genes. Plasmodium lactate dehydrogenase (pLDH)-based tests are promising alternatives, but less available. This study assessed the performances of HRP2 and pLDH(pan) tests under field conditions.

METHODS

The study performed a prospective facility-based diagnostic evaluation of two malaria RDTs in Aweil, South Sudan, during the high transmission season. Capillary blood by fingerprick was collected from 800 children under 15 years of age with fever and no signs of severity. SD Bioline HRP2 and CareStart pLDH(pan) RDTs were performed in parallel, thick and thin smears for microscopy were examined, and dried blood was used for PCR testing.

RESULTS

Using microscopy as the gold standard, the sensitivity of both tests was estimated at  > 99%, but the specificity of each was lower: 55.0% for the pLDH test and 61.7% for the HRP2 test. When using PCR as the gold standard, the sensitivity of both tests was lower than the values assessed using microscopy (97.0% for pLDH and 96.5% for HRP2), but the specificity increased (65.1% for pLDH and 72.9% for HRP2). Performance was similar across different production lots, sex, and age. Specificity of both the pLDH and HRP2 tests was significantly lower in children who reported taking a therapeutic course of anti-malarials in the 2 months prior to enrollment. The prevalence of pfhrp2/3 deletions in the study population was 0.6%.

CONCLUSIONS

The low specificity of the pLDH RDT in this setting confirms previous results and suggests a problem with this specific test. The prevalence of pfhrp2/3 deletions in the study area warrants continued monitoring and underscores the relevance of assessing deletion prevalence nationally. Improved malaria RDTs for high-transmission environments are needed.

摘要

背景

快速诊断检测(RDT)是撒哈拉以南非洲疟疾诊断的主要工具,但由于成功治疗疟疾后阳性持续时间较长,最常用的富含组氨酸蛋白 2(HRP2)抗原检测在高传播环境中的实用性有限。HRP2 检测也受到不携带 pfhrp2 或 pfhrp3 基因的疟原虫的威胁。基于乳酸脱氢酶(pLDH)的检测是有前途的替代品,但供应较少。本研究在高传播季节在南苏丹的 Aweil 进行了一项现场条件下的 HRP2 和 pLDH(泛)检测的前瞻性现场评估。通过指尖采集了 800 名 15 岁以下发热且无严重症状的儿童的毛细血管血。同时进行了 SD Bioline HRP2 和 CareStart pLDH(泛)RDT 检测,并行进行了厚、薄血涂片显微镜检查,并使用干血进行 PCR 检测。

结果

以显微镜检查为金标准,两种检测方法的敏感性均估计超过 99%,但每种方法的特异性较低:pLDH 检测为 55.0%,HRP2 检测为 61.7%。当使用 PCR 作为金标准时,两种检测方法的敏感性均低于使用显微镜评估的值(pLDH 为 97.0%,HRP2 为 96.5%),但特异性增加(pLDH 为 65.1%,HRP2 为 72.9%)。不同生产批次、性别和年龄的性能相似。在报告在入组前 2 个月内接受抗疟治疗疗程的儿童中,pLDH 和 HRP2 检测的特异性均显著降低。研究人群中 pfhrp2/3 缺失的流行率为 0.6%。

结论

在这种情况下,pLDH RDT 的低特异性证实了之前的结果,并表明该特定检测存在问题。研究区域中 pfhrp2/3 缺失的流行率需要持续监测,并强调了在全国范围内评估缺失流行率的相关性。需要开发用于高传播环境的改进型疟疾 RDT。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/78cf/9461093/543155a2bcd2/12936_2022_4280_Fig1_HTML.jpg

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