TY - JOUR
T1 - Human papillomavirus typing with a polymerase chain reaction-based genotyping array compared with type-specific PCR
AU - Lin, Ching Yu
AU - Chao, Angel
AU - Yang, Yuh Cheng
AU - Chou, Hung Hsueh
AU - Ho, Chih Ming
AU - Lin, Ruey Wen
AU - Chang, Ting Chang
AU - Chiou, Jia Yia
AU - Chao, Fang Yu
AU - Wang, Kung Liahng
AU - Chien, Tsai Yen
AU - Hsueh, Swei
AU - Huang, Chu Chun
AU - Chen, Chien Jen
AU - Lai, Chyong Huey
N1 - Funding Information:
The King Car Research Foundation of the King Car Food Industrial Co. Ltd. supported this work.
PY - 2008/8
Y1 - 2008/8
N2 - Background: Type-specific persistence of human papillomavirus (HPV) infection can cause invasive cervical cancer. Objectives: To evaluate the efficacy of HPV detection and typing with a general polymerase chain reaction (PCR)-based genotyping array and to compare it with a type-specific PCR assay. Study design: Four hundred and thirty-three cervical samples were tested with a modified MY11/GP6+ PCR-based reverse-blot assay (EasyChip® HPV Blot; King Car, Taiwan [hereafter HPV Blot]) and with 20 genotypes of L1-type-specific PCR (HPV-6, -11, -16, -18, -31, -33, -35, -39, -45, -51, -52, -53, -56, -58, -59, -62, -66, -68, -70, and -71 [CP8061]). Results: The concordance of the two tests in determining HPV positivity was 96.8% (419/433), with a Cohen's κ = 0.93 (95% CI: 0.90-0.97) and McNemar's test of P = 1.0, which indicates excellent agreement. The overall concordance of the two tests in the identification of type-specific HPV was 91.0% (394/433). Sensitivity (90-100%), specificity (99.2-100%), and accuracy (98.6-100%) rates of HPV Blot against the gold standard were satisfactory for HPV-16, -18, -58, -33, -52, -39, -45, -31, -51, -70 while HPV-71 (63.6%) had suboptimal sensitivity. Though the κ values between the two tests for many individual genotypes could not be reliably calculated because of low positivity, the κ values for HPV-16, -52, and -58 were excellent (0.93, 0.96, and 0.95, respectively). Conclusion: The modified MY11/GP6+ PCR-based HPV Blot assay is accurate and sensitive for detection and genotyping of HPV in cervical swab samples.
AB - Background: Type-specific persistence of human papillomavirus (HPV) infection can cause invasive cervical cancer. Objectives: To evaluate the efficacy of HPV detection and typing with a general polymerase chain reaction (PCR)-based genotyping array and to compare it with a type-specific PCR assay. Study design: Four hundred and thirty-three cervical samples were tested with a modified MY11/GP6+ PCR-based reverse-blot assay (EasyChip® HPV Blot; King Car, Taiwan [hereafter HPV Blot]) and with 20 genotypes of L1-type-specific PCR (HPV-6, -11, -16, -18, -31, -33, -35, -39, -45, -51, -52, -53, -56, -58, -59, -62, -66, -68, -70, and -71 [CP8061]). Results: The concordance of the two tests in determining HPV positivity was 96.8% (419/433), with a Cohen's κ = 0.93 (95% CI: 0.90-0.97) and McNemar's test of P = 1.0, which indicates excellent agreement. The overall concordance of the two tests in the identification of type-specific HPV was 91.0% (394/433). Sensitivity (90-100%), specificity (99.2-100%), and accuracy (98.6-100%) rates of HPV Blot against the gold standard were satisfactory for HPV-16, -18, -58, -33, -52, -39, -45, -31, -51, -70 while HPV-71 (63.6%) had suboptimal sensitivity. Though the κ values between the two tests for many individual genotypes could not be reliably calculated because of low positivity, the κ values for HPV-16, -52, and -58 were excellent (0.93, 0.96, and 0.95, respectively). Conclusion: The modified MY11/GP6+ PCR-based HPV Blot assay is accurate and sensitive for detection and genotyping of HPV in cervical swab samples.
KW - Agreement
KW - HPV Blot
KW - Human papillomavirus
KW - Type-specific PCR
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U2 - 10.1016/j.jcv.2008.03.018
DO - 10.1016/j.jcv.2008.03.018
M3 - Article
C2 - 18455959
AN - SCOPUS:46149088452
SN - 1386-6532
VL - 42
SP - 361
EP - 367
JO - Journal of Clinical Virology
JF - Journal of Clinical Virology
IS - 4
ER -