Performance of the Amplicor human immunodeficiency virus type 1 PCR and analysis of specimens with false-negative results

Barlow, Katrina L.; Tosswill, Jennifer; Parry, John; Clewley, Jonathan P.

doi:10.1128/jcm.35.11.2846-2853.1997

Cited by 53 publications

(10 citation statements)

References 30 publications

(54 reference statements)

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“…Consequently, the detection of viral variants is a concern for NAT. 21 In this study, the TMA duplex assay detected with similar efficiency the calibrated reference strains of HIV-1 subtype B and HCV genotype 1, in addition to clinical samples of HIV-1 subtypes A-E and HCV subtypes 1a-4a of various geographical origins ( Table 1).…”

Section: Discussionsupporting

confidence: 59%

Evaluation of a transcription‐mediated amplification‐based HCV and HIV‐1 RNA duplex assay for screening individual blood donations: a comparison with a minipool testing system

et al. 2003

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Section: Discussionsupporting

confidence: 59%

Evaluation of a transcription‐mediated amplification‐based HCV and HIV‐1 RNA duplex assay for screening individual blood donations: a comparison with a minipool testing system

et al. 2003

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“…At low virus amounts, the background may completely hide the signal generated by the target. If that happens, then assays produce false-negative results (3,27). Of course, the MCT format cannot eliminate background synthesis; however, because of the high resolving power of the MCT gel, it could negate that effect by spatially separating background colonies from those produced by the target.…”

Section: Effects Of Background Synthesismentioning

confidence: 99%

Molecular Colony Diagnostics: Detection and Quantitation of Viral Nucleic Acids by In-Gel PCR

et al. 2002

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When PCR is carried out in a polyacrylamide gel, each target molecule forms a molecular colony that comprises many copies of the original template. By counting the number of colonies, one can directly determine the target titer, with 100% of the DNA molecules and approximately 15% of the RNA molecules being detected. Furthermore, because of the spatial separation of the products in the gel, no interference is observedfrom another simultaneously amplified target even if it is present at a 106 higher amount orfrom human nucleic acids that outweigh the target by up to a factor of 1,012, which is often true of clinical samples. All these features provide for an accurate and reliable assay of viruses even at very low amounts, that is, in cases most important to diagnostics.

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“…To enhance the level of detection, we performed kinetic studies with samples with ODs higher than the average of the negative control ODs but lower than the threshold (average negative control ODs ϩ standard deviations). We carried out these studies with different incubation times (4,8,16,24,36, and 48 h). More than 50% of the samples became positive when the incubation period reached 16 h (plateau at 16 h).…”

Section: Discussionmentioning

confidence: 99%

Comparison of an Amplified Enzyme-Linked Immunosorbent Assay with Procedures Based on Molecular Biology for Assessing Human Immunodeficiency Virus Type 1 Viral Load

Goldschmidt¹,

Ait-Arkoub²,

Aubin³

1998

Clin Diagn Lab Immunol

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The sensitivity of the enzyme-linked amplified sorbent test (ELAST) was compared with those of other classic enzyme-linked immunosorbent assays (ELISAs), with or without previous acidic immunocomplex dissociation (ICD), in a series of samples at different stages of human immunodeficiency virus type 1 (HIV-1) infection. The limit of viral detection of ELAST was assessed with fresh HIV-1 preparations quantified by reverse transcription-PCR and with the P24 antigen (Ag) Sanofi Pasteur Calibrator containing lyophilized virus. The P24 Ag detection capacity of ELAST was compared with that of NASBA in samples obtained from infected subjects with less than 250 CD4+ cells. The results of the present study show that ELAST was the most sensitive method for detecting P24 Ag compared to classic ELISA and ICD plus ELISA. ELAST was able to detect 0.5 pg of P24 Ag per ml in a whole virus preparation and the equivalent of 330 to 1,000 RNA copies/ml of HIV. The rate of detection of P24 Ag was always higher in subjects with low levels of anti-P24 antibodies. The number of positive results was dramatically enhanced (from 37% to 94% for subjects with <250 CD4+ cells) when the incubation period was prolonged from 1 to 16 h. In a third series of 84 samples (<250 CD4+ cells) tested in parallel, NASBA yielded 83% of the positive results and ELAST yielded 79%. Considering the high sensitivity, low cost, simplicity of equipment (only a plate reader), and possibility for full automation, ELAST appears to be a promising new tool for measuring viral load, especially in areas with few resources, in which the procedures based on molecular biology techniques may be difficult to install.

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Performance of the Amplicor human immunodeficiency virus type 1 PCR and analysis of specimens with false-negative results

Cited by 53 publications

References 30 publications

Evaluation of a transcription‐mediated amplification‐based HCV and HIV‐1 RNA duplex assay for screening individual blood donations: a comparison with a minipool testing system

Evaluation of a transcription‐mediated amplification‐based HCV and HIV‐1 RNA duplex assay for screening individual blood donations: a comparison with a minipool testing system

Molecular Colony Diagnostics: Detection and Quantitation of Viral Nucleic Acids by In-Gel PCR

Comparison of an Amplified Enzyme-Linked Immunosorbent Assay with Procedures Based on Molecular Biology for Assessing Human Immunodeficiency Virus Type 1 Viral Load

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