| Literature DB >> 24040090 |
Adrienne Trombley Hall1, Ashley McKay Zovanyi, Deanna Rose Christensen, Jeffrey William Koehler, Timothy Devins Minogue.
Abstract
Polymerase chain reaction (PCR) is commonly used for pathogen detection in clinical and environmental samples. These sample matrices often contain inhibitors of PCR, which is a primary reason for sample processing; however, the purification process is highly inefficient, becoming unacceptable at lower signature concentrations. One potential solution is direct PCR assessment without sample processing. Here, we evaluated nine inhibitor-resistant PCR reagents for direct detection of Francisella tularensis in seven different clinical and environmental samples using an established real-time PCR assay to assess ability to overcome PCR inhibition. While several of these reagents were designed for standard PCR, the described inhibitor resistant properties (ex. Omni Klentaq can amplify target DNA samples of up to 20% whole blood or soil) led to our evaluation with real-time PCR. A preliminary limit of detection (LOD) was determined for each chemistry in whole blood and buffer, and LODs (20 replicates) were determined for the top five chemistries in each matrix (buffer, whole blood, sputum, stool, swab, soil, and sand). Not surprisingly, no single chemistry performed the best across all of the different matrices evaluated. For instance, Phusion Blood Direct PCR Kit, Phire Hot Start DNA polymerase, and Phire Hot Start DNA polymerase with STR Boost performed best for direct detection in whole blood while Phire Hot Start DNA polymerase with STR Boost were the only reagents to yield an LOD in the femtogram range for soil. Although not the best performer across all matrices, KAPA Blood PCR kit produced the most consistent results among the various conditions assessed. Overall, while these inhibitor resistant reagents show promise for direct amplification of complex samples by real-time PCR, the amount of template required for detection would not be in a clinically relevant range for most matrices.Entities:
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Year: 2013 PMID: 24040090 PMCID: PMC3767612 DOI: 10.1371/journal.pone.0073845
Source DB: PubMed Journal: PLoS One ISSN: 1932-6203 Impact factor: 3.240
Description of each chemistry tested with .
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| Ampdirect | Rockland Immunochemicals | Buffer | Neutralizes inhibitory substances in human blood for direct DNA amplification. |
| Phire Hot Start DNA Polymerase | Finnzymes/New England Biolabs | Buffer plus polymerase | The enhanced polymerase enables short extension times, improved yields, and amplifies long DNA fragments. |
| Omni Klentaq | DNA Polymerase Technology | Polymerase | Overcomes inhibitors in 20% whole blood or crude soil samples. |
| Phusion Blood Direct PCR Kit | Finnzymes/New England Biolabs | Buffer plus polymerase | Designed to perform PCR directly from whole blood with no prior DNA extraction. |
| KAPA Blood PCR Kit | KAPA Biosystems | Buffer plus polymerase | Amplification of DNA fragments directly from whole blood. |
| Hemo KlenTaq | New England Biolabs | Buffer plus polymerase | N-terminal (280 amino acid) truncation and mutations allow resistance to inhibitors for direct amplification in whole blood. |
| PCRboost | Biomatrica | Buffer | Improves amplification of low copy transcripts, degraded, trace, or inhibitory samples. |
| STRboost | Biomatrica | Buffer | For use with limited, degraded, and blood samples. |
| Terra PCR Direct Polymerase Mix | Clontech | Buffer plus polymerase | Direct amplification from tissue samples, crude extracts, and dirty templates. |
Description of the real-time PCR curve scoring.
| Qualitative score | Positive characteristics | Negative characteristics |
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| 1 | a. Sample detection – software based Cq determination | a. Background fluorescence continuously decreases below starting levels with jagged readings (>1 RFU change) |
| b. Amplification curves are not sigmoidal | ||
| c. Endpoint fluorescence is inconsistent | ||
| d. Replicate curves are not parallel, and the Cq values vary (>1 Cq difference) | ||
| 2 | a. All characteristics in 1 b. Amplification curves are sigmoidal | a. Background fluorescence continuously decreases below starting levels (>1 RFU change) |
| b. Endpoint fluorescence is inconsistent | ||
| c. Replicate curves are not parallel but maintain similar Cq values (1-2 Cq difference) | ||
| 3 | a. All characteristics in 2 | a. Background fluorescence is rough with jagged readings |
| b. End point fluorescence remains consistent | b. Replicate curves have some separation with similar Cq values (<1 Cq difference) | |
| 4 | a. All characteristics in 3 | a. Background fluorescence has some inconsistency |
| b. Replicate curves are parallel with very similar Cq values (<1 Cq difference) | ||
| 5 | a. All characteristics in 4 | |
| b. Background fluorescence remains smooth and consistent (<1 RFU difference) |
Preliminary LOD determination (2/2) using FT-MM across each matrix.
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| Whole blood | 2.5% | ND |
| 0.5% | 0.02 pg | |
| 0.25% | 0.01 pg | |
| 0.05% | 0.01 pg | |
| Sputum | 2.5% | 10 pg |
| 0.5% | 0.2 pg | |
| 0.25% | 1 pg | |
| 0.05% | 0.02 pg | |
| Swab | 25% | 0.01 pg |
| 5% | 0.01 pg | |
| Stool | 2.5% | 0.01 pg |
| 0.5% | 0.002 pg | |
| Soil | 0.25% | ND |
| 0.05% | ND | |
| 0.025% | 0.01 pg | |
| 0.005% | 0.01 pg | |
| Sand | 2.5% | ND |
| 0.5% | 0.02 pg | |
| 0.25% | 0.01 pg | |
| 0.05% | 0.01 pg |
ND, not detected at any DNA concentration
Comparison of inhibitor-resistant polymerases with and without Taq DNA polymerase addition in buffer.
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| Phire | 10 pg | 31.74 | 2 | 0.050 pg | 36.42 | 4 | |
| Omni Klentaq | 0.01 pg | 35.63 | 4 | 0.050 pg | 31.75 | 3 | |
| Phusion | 0.01 pg | 38.1 | 4 | 0.01 pg | 37.73 | 5 | |
| KAPA | 0.01 pg | 32.05 | 4 | 0.01 pg | 34.74 | 5 | |
| Hemo KlenTaq | 0.01 pg | 37.65 | 1 | 0.01 pg | 35.04 | 2 | |
| Terra PCR Direct | ND | - | 0 | 100 pg | 33.66 | 2 | |
See Table 2 for real-time PCR Score description
Cq values represent average Cq value across two replicates
ND, not detected at any DNA concentration
Impact of inhibitor-resistant reagents on detection and qualitative real-time PCR characteristics.
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| Ampdirect | 0.01 pg | 5 | ND | 0.01 pg | 10 pg | 0.2pg | 1 (0.5%) | |
| Phire | 0.050 pg | 4 | 0.05 pg | 0.01 pg | 0.050 pg | 0.01 pg | 2 (0.5%) | |
| Omni Klentaq | 0.050 pg | 2 | 10 pg | ND | ND | 0.2 pg | 1 (0.05%) | |
| Phusion | 0.01 pg | 5 | 0.01 pg | 0.01 pg | 0.050 pg | 0.01 pg | 2 (0.5%) | |
| KAPA | 0.01 pg | 3 | 0.1 pg | 0.01 pg | 0.050 pg | 0.02 pg | 1 (0.5%) | |
| Hemo KlenTaq | 0.050 pg | 3 | ND | 0.002 pg | ND | 0.01 pg | 1 (0.5%) | |
| PCRboost | 0.01 pg | 5 | ND | ND | 1 pg | 0.2 pg | 3 (0.05%) | |
| STRboost | 0.01 pg | 5 | ND | ND | 0.1 pg | 0.02 pg | 3 (0.05%) | |
| Terra PCR Direct | 0.01 pg | 2 | ND | ND | ND | ND | ND | |
| FT-MM | 0.01 pg | 5 | ND | ND | ND | 0.01 pg | 3 (0.05%) | |
| Phire plus Ampdirect | 0.01 pg | 5 | 0.050 pg | 0.01 pg | 0.01 pg | 0.002 pg | 2 (0.5%) | |
| Phire plus STRboost | 0.01 pg | 5 | 0.1 pg | 0.02 pg | 0.050 pg | 0.02 pg | 3 (0.5%) | |
| Phire plus PCRboost | 0.01 pg | 4 | 0.050 pg | 0.02 pg | 0.050 pg | 0.02 pg | 2 (0.05%) | |
See Table 2 for real-time PCR Score description
2/2 replicates had to be positive for the limit of detection call
ND, not detected at any DNA concentration
Preliminary estimation of LOD down-selected inhibitor-resistant reagents for sputum, stool, soil, sand, and swab.
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| Sputum | 2.50% | ND | 0.050 pg | 0.1 pg | 1 pg | 1 pg |
| 0.50% | 0.2 pg | 0.01 pg | 0.02 pg | 0.2 pg | 0.2 pg | |
| Stool | 25% | ND | ND | ND | ND | ND |
| 5% | 0.02 pg | 0.1 pg | 0.01 pg | 0.01 pg | 0.01 pg | |
| 2.50% | 0.01 pg | 0.050 pg | 0.01 pg | 0.01 pg | 0.01 pg | |
| 0.50% | 0.01 pg | 0.002 pg | 0.01 pg | 0.002 pg | 0.01 pg | |
| Soil | 0.25% | ND | ND | ND | ND | ND |
| 0.05% | 0.01 pg | 0.2 pg | 0.02 pg | 0.01 pg | 0.2 pg | |
| Sand | 2.50% | 0.050 pg | 0.050 pg | 0.01 pg | 1 pg | ND |
| 0.50% | 0.2 pg | 0.01 pg | 0.02 pg | 0.02 pg | 2 pg | |
| 0.25% | 0.01 pg | 0.01 pg | 0.01 pg | 0.050 pg | 1 pg | |
| 0.05% | 0.2 pg | 0.01 pg | 0.01 pg | 0.01 pg | 0.01 pg | |
| Swab | 25% | 0.01 pg | 1 pg | 0.01 pg | 0.01 pg | 0.050 pg |
| 5% | 0.01 pg | 0.01 pg | 0.002 pg | 0.01 pg | 0.02 pg |
2/2 replicates had to be positive for the limit of detection call
ND, not detected at any DNA concentration
Limits of detection (20/20) for each matrix.
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| Phusion | Whole blood | 0.5% | 0.2 pg | 28.11 ± 3.32 | 11.81 |
| Sputum | 0.5% | 0.2 pg | 35.11 ± 0.38 | 1.09 | |
| Stool | 5% | 0.02 pg | 37.18 ± 1.72 | 4.62 | |
| Soil | 0.05% | 2 pg | 32.08 ±1.22 | 3.82 | |
| Sand | 2.5% | 0.1 pg | 35.07 ± 0.42 | 1.20 | |
| Swab | 25% | 0.05 pg | 34.19 ± 0.33 | 0.97 | |
| Phire | Whole blood | 0.5% | 0.2 pg | 28.90 ±3.70 | 12.82 |
| Sputum | 0.5% | 0.2 pg | 36.80 ± 1.01 | 2.74 | |
| Stool | 2.5% | 0.05 pg | 35.25 ± 0.55 | 1.56 | |
| Soil | 0.05% | 2 pg | ND for 15/20 | - | |
| Sand | 2.5% | 0.1 pg | 37.02 ± 1.45 | 3.91 | |
| Swab | 5% | 0.02 pg | 35.08 ± 0.59 | 1.67 | |
| KAPA | Whole blood | 0.5% | 0.2 pg | 31.28 ± 3.51 | 11.22 |
| Sputum | 0.5% | 0.2 pg | 33.92 ± 0.19 | 0.57 | |
| Stool | 5% | 0.02 pg | 34.61 ± 0.62 | 1.78 | |
| Soil | 0.05% | 0.2 pg | 32.60 ± 0.31 | 0.96 | |
| Sand | 2.5% | 0.05 pg | 35.09 ± 0.46 | 1.32 | |
| Swab | 25% | 0.05 pg | 33.31 ± 0.26 | 0.79 | |
| Phire plus | Whole blood | 0.5% | 0.2 pg | 23.05 ± 7.73 | 33.54 |
| Ampdirect | Sputum | 0.5% | 0.2 pg | 35.33 ± 0.68 | 1.94 |
| Stool | 5% | 0.02 pg | 35.20 ± 1.77 | 5.02 | |
| Soil | 0.05% | 0.2 pg | 32.36 ± 0.51 | 1.59 | |
| Sand | 0.05% | 0.2 pg | 34.13 ± 0.60 | 1.77 | |
| Swab | 25% | 0.1 pg | 33.06 ± 0.41 | 1.24 | |
| Phire plus | Whole blood | 0.5% | 0.2 pg | 32.28 ± 0.56 | 1.72 |
| STRboost | Sputum | 0.5% | 0.2 pg | 34.40 ± 0.67 | 1.94 |
| Stool | 5% | 0.02 pg | 35.00 ± 0.91 | 2.60 | |
| Soil | 0.05% | 0.2 pg | 30.03 ± 0.36 | 1.20 | |
| Sand | 0.5% | 0.2 pg | 34.18 ± 0.81 | 2.38 | |
| Swab | 25% | 0.05 pg | 33.60 ± 0.39 | 1.17 |
ND, not detectable
19/20 replicates were positive