TY - JOUR
KW - Mycobacterium leprae
KW - NGS
KW - RLEP
KW - in-house reference DNA
KW - Molecular diagnosis
KW - next-generation sequencing
KW - quantitative PCR
AU - Girma S
AU - Gemeda M
AU - Woldesemayat A
AU - Bobosha K
AU - Gadisa E
AB - <p><strong>INTRODUCTION: </strong></p>

<p>To develop an in-house reference control DNA standard targeting the RLEP region of Mycobacterium leprae for use in quantitative polymerase chain reaction (qPCR) diagnostics, aiming to reduce dependence on animal models and external sources.</p>

<p><strong>METHOD: </strong></p>

<p>Previously characterized DNA samples from patients with leprosy were used to amplify and sequence the 450-base pair RLEP region. A specific 131-base pair segment within this region was targeted for qPCR assay development. The amplified products were purified; sequenced using Illumina next-generation sequencing technology; and validated through bioinformatics analyses, including Basic Local Alignment Search Tool (BLAST; National Institutes of Health) alignment and copy number assessment.</p>

<p><strong>RESULTS: </strong></p>

<p>The consensus sequence aligned perfectly with the known RLEP region. The BLAST analysis revealed 37 copies of the target sequence throughout the genome, confirming the sequence's utility as a sensitive diagnostic marker. The qPCR assay successfully detected the target in both reference and clinical samples, with melting curve analysis indicating high specificity.</p>

<p><strong>DISCUSSION: </strong></p>

<p>An in-house M leprae RLEP control standard was successfully developed that provides a reliable, ethical, and resource-efficient alternative to traditional animal-derived controls for leprosy diagnosis using qPCR.</p>

BT - Laboratory medicine
C1 - https://www.ncbi.nlm.nih.gov/pubmed/42057581
DA - 04/2026
DO - 10.1093/labmed/lmag020
IS - 3
J2 - Lab Med
LA - ENG
M3 - Article 
N2 - <p><strong>INTRODUCTION: </strong></p>

<p>To develop an in-house reference control DNA standard targeting the RLEP region of Mycobacterium leprae for use in quantitative polymerase chain reaction (qPCR) diagnostics, aiming to reduce dependence on animal models and external sources.</p>

<p><strong>METHOD: </strong></p>

<p>Previously characterized DNA samples from patients with leprosy were used to amplify and sequence the 450-base pair RLEP region. A specific 131-base pair segment within this region was targeted for qPCR assay development. The amplified products were purified; sequenced using Illumina next-generation sequencing technology; and validated through bioinformatics analyses, including Basic Local Alignment Search Tool (BLAST; National Institutes of Health) alignment and copy number assessment.</p>

<p><strong>RESULTS: </strong></p>

<p>The consensus sequence aligned perfectly with the known RLEP region. The BLAST analysis revealed 37 copies of the target sequence throughout the genome, confirming the sequence's utility as a sensitive diagnostic marker. The qPCR assay successfully detected the target in both reference and clinical samples, with melting curve analysis indicating high specificity.</p>

<p><strong>DISCUSSION: </strong></p>

<p>An in-house M leprae RLEP control standard was successfully developed that provides a reliable, ethical, and resource-efficient alternative to traditional animal-derived controls for leprosy diagnosis using qPCR.</p>

PY - 2026
T2 - Laboratory medicine
TI - Development of an in-house control standard for quantitative polymerase chain reaction-based diagnosis of leprosy.
VL - 57
SN - 1943-7730
ER -