Epidemiological serosurvey of chikungunya fever post outbreak at Tanjung Sepat, Malaysia

Khor, Chee‐Sieng; Teoh, Boon‐Teong; Sam, Sing‐Sin; Khoo, Hooi-Yuen; Azizan, Noor-Syahida; CheMatSeri, AsmaAnati; Chin, Kim-Ling; Hamim, Zur-Raiha; Mohamed-Romai-Noor, Noor-Adila; Yaacob, Che-Norainon; Abd-Jamil, Juraina; Lee, Hai Yen; Soh, Yih-Harng; AbuBakar, Sazaly

doi:10.3855/jidc.16613

Cited by 1 publication

(1 citation statement)

References 30 publications

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“…The CHIKV was then imported from Myanmar into its adjacent country, Yunnan Province, China in 2019 (Yin et al, 2021). In Malaysia, CHIKV re-emerged in 2019 after a 10-year gap following the previous outbreak from 2008 to 2009 (Sam et al, 2009;Ministry of Health Malaysia, 2022;Khor et al, 2023).…”

Section: Introductionmentioning

confidence: 99%

A TaqMan minor groove binder probe-based quantitative reverse transcription polymerase chain reaction for detection and quantification of chikungunya virus

Y.Z.

2023

Trop Biomed

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Chikungunya virus (CHIKV) is a mosquito-borne alphavirus with widespread distribution across the globe. Since 2016, CHIKV re-emerged in several countries including Indian subcontinent and Southeast Asia. A proper diagnostic tool for early diagnosis of CHIKV infection is crucial to facilitate patient management and control virus transmission at the earliest stage of outbreak. Therefore, a TaqMan minor groove binder (MGB) probe-based quantitative reverse transcription polymerase chain reaction (qRT-PCR) assay was developed to detect and quantify the CHIKV. The primers and probe were designed based on a conserved genomic region of 730 global CHIKV sequences that is located between nsP1 and nsP2 genes. The nucleotide mismatches of primers and probe with 730 global CHIKV sequences and 13 alphaviruses were then analysed in silico. In this study, the last 5 nucleotides at 3' end of primers and 5' end of probe were considered to be the critical regions for priming. In silico analysis revealed that the critical regions of primers and probe were at least 99.6% matched with the 730 global CHIKV sequences. Besides, the primers and probe showed at least 5/20 (25.0%) and 4/17 (23.5%) nucleotide mismatches with 13 alphaviruses respectively. The amplification efficiency of qRT-PCR assay was 100.59% (95% CI= 93.06, 109.33) with a R 2 score of 0.957. Its limit of detection (LOD) at 95% probability level was 16.6 CHIKV RNA copies (95% CI= 12.9, 28.9). The qRT-PCR assay was specific to CHIKV without cross-reacting with all dengue virus serotypes, Getah virus, Tembusu virus and Zika virus. The diagnostic results of qRT-PCR assay were perfectly agreed (k=1.000, p=0.003) with a commercial trioplex assay, with sensitivity of 100% (95% CI= 61, 100) and specificity of 100% (95% CI= 44, 100). Overall, the developed qRT-PCR assay is ideal for rapid, sensitive and specific detection as well as quantification of CHIKV.

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Section: Introductionmentioning

confidence: 99%

A TaqMan minor groove binder probe-based quantitative reverse transcription polymerase chain reaction for detection and quantification of chikungunya virus

Y.Z.

2023

Trop Biomed

View full text Add to dashboard Cite

show abstract

Epidemiological serosurvey of chikungunya fever post outbreak at Tanjung Sepat, Malaysia

Cited by 1 publication

References 30 publications

A TaqMan minor groove binder probe-based quantitative reverse transcription polymerase chain reaction for detection and quantification of chikungunya virus

A TaqMan minor groove binder probe-based quantitative reverse transcription polymerase chain reaction for detection and quantification of chikungunya virus

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