| Literature DB >> 29425193 |
Dora Buonfrate1, Ana Requena-Mendez2, Andrea Angheben1, Michela Cinquini3, Mario Cruciani4, Andrea Fittipaldo3, Giovanni Giorli1, Federico Gobbi1, Chiara Piubelli1, Zeno Bisoffi1.
Abstract
BACKGROUND: Strongyloides stercoralis infection is a neglected tropical disease which can lead to severe symptoms and even death in immunosuppressed people. Unfortunately, its diagnosis is hampered by the lack of a gold standard, as the sensitivity of traditional parasitological tests (including microscopic examination of stool samples and coproculture) is low. Hence, alternative diagnostic methods, such as molecular biology techniques (mostly polymerase chain reaction, PCR) have been implemented. However, there are discrepancies in the reported accuracy of PCR.Entities:
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Year: 2018 PMID: 29425193 PMCID: PMC5823464 DOI: 10.1371/journal.pntd.0006229
Source DB: PubMed Journal: PLoS Negl Trop Dis ISSN: 1935-2727
Fig 1Study flow chart.
Main characteristics of the study sets included in the analysis.
| Study | Index test(s) and PCR target | Reference test(s) | Setting | Population |
|---|---|---|---|---|
| Ahmad 2013[ | Nested PCR | Serology | Endemic country | All ages |
| Amor 2016[ | Real-time PCR | Baermann | Endemic country | Children |
| Becker 2015_a [ | Real-time PCR | Combination of parasitological methods | Endemic country | All ages |
| Becker 2015_b[ | Real-time PCR | Combination of parasitological methods | Endemic country | All ages |
| Buonfrate 2017_a[ | Real-time PCR | APC | Non endemic country | Adults |
| Buonfrate 2017_b[ | Real-time PCR | Serology | Non endemic country | Adults |
| De Paula 2015_a [ | Conventional | APC | Endemic country | Not specified |
| De Paula 2015_b[ | Real-time PCR | APC | Endemic country | Not specified |
| Knopp 2014[ | Real-time PCR | Baermann | Endemic country | All ages |
| Lohd 2016[ | Conventional PCR | Combination of parasitological methods | Endemic country | All ages |
| Meurs 2017[ | Real-time PCR | Combination of parasitological methods | Endemic country | All ages |
| Shar 2013[ | Real-time PCR | Combination of parasitological methods | Endemic country | Children |
| Sharifdini 2015_a[ | Nested | Combination of parasitological methods | Endemic country | Not specified |
| Sharifdini 2015_b[ | Real-time PCR | Combination of parasitological methods | Endemic country | Not specified |
| Sultana 2013[ | Real-time PCR | APC | Endemic country | Not specified |
| Ten Hove 2009[ | Real-time PCR | Baermann | Non endemic country | Adults |
| Verweij 2009[ | Real-time PCR | Combination of parasitological methods | Endemic country | All ages |
| Zueter 2014[ | Real-time PCR | Serology | Endemic country | Adults |
ITS1 = Internal transcribed spacer 1
rRNA = ribosomal RNA
Fig 2Risk of bias and applicability concerns summary.
Fig 3Risk of bias and applicability concerns graph.
Fig 4Forest plot showing the accuracy of the molecular techniques according to the single study sets.
Summary estimates of diagnostic accuracy of PCR techniques for the diagnosis of Strongyloides stercoralis infection.
| Reference Test | All PCRs | Real Time PCR | ||
|---|---|---|---|---|
| Serology or parasitological methods | Estimate (95% CI) | S.E. | Estimate (95% CI) | S.E. |
| Sensitivity | 61.85% (42.0–78.4) | 9.70 | 56.50% (39.2–72.4) | 8.79 |
| Specificity | 95.27% (92.0–97.2) | 1.28 | 95.38% (91.7–97.5) | 1.40 |
| DOR | 32.7 (15.3–70.0) | 12.6 | 26.8 (13.2–54.8) | 9.77 |
| LR+ | 13.1 (8.0–21.3) | 3.2 | 12.2 (7.1–21.0) | 3.38 |
| LR- | 0.40 (0.24–0.65) | 0.09 | 0.45 (0.31–0.67) | 0.08 |
| 1/LR- | 2.5 (1.53–4.06) | 0.62 | 2.2 (1.49–3.22) | 0.43 |
| Sensitivity | 71.76% (52.23–85.52) | 8.72 | 64.42% (46.2–77.7) | 8.31 |
| Specificity | 93.46% (90.35–95.61) | 1.32 | 93.93% (90.3–96.3) | 1.49 |
| DOR | 36.3 (15.4–85.4) | 15.8 | 26.8 (12.7–56.6) | 10.21 |
| LR+ | 10.9 (7.2–16.6) | 2.31 | 10.4 (6.4–16.8) | 2.55 |
| LR- | 0.30 (0.16–0.55) | 0.09 | 0.4 (0.25–0.60) | 0.09 |
| 1/LR- | 3.3 (1.49–3.22) | 1.01 | 2.6 (1.66–3.98) | 0.57 |
PCR, polymerase chain reaction; S.E., standard error; DOR, diagnostic odds ratio; LR, likelihood ratio
Estimates and S.Es for sensitivity and specificity are here reported in %.
a Studies included conventional PCR, nested PCR, real-time PCR
Either Baermann method, agar plate culture, Harada-Mori culture, or a combination of fecal methods
Fig 5Accuracy of all PCR techniques (comparison with both fecal and serological tests): ROC curve.
Fig 6Accuracy of real-time PCR (comparison with fecal tests): ROC curve.
Of note, the only study using a CRS (including serology) to assess the accuracy of real-time PCR demonstrated a sensitivity of 56.8%[20], which is almost the same value found with the meta-analysis. On the other hand, the only study using a Bayesian approach [11] demonstrated an extremely low sensitivity (11.6%) of real-time PCR.
Summary of findings table for the review of PCR techniques for the diagnosis of Strongyloides stercoralis infection.
| Interpretative criteria to define: Index vs. Reference Test | ||||
|---|---|---|---|---|
| 17 | 21.1% | Assuming (based on the mean prevalence) 21 out of 100 patients with SSI, eight would be missed by a single PCR test (38% of 21). Of the 79 patients without SSI, four (5%) would have a false positive result of the PCR test. | ||
| 14 | 18.5% | Assuming 18 out of 100 patients with SSI, five would be missed by a single PCR test. Of the 82 patients without SSI, five would have a false positive result of the PCR test. | ||
| 14 | 20.5% | Assuming 20 out of 100 patients with SSI, nine would be missed by a single PCR test. Of the other 80, four will have a false positive result of the PCR test. | ||
| 12 | 20.3% | Assuming 20 out of 100 patients with SSI, seven would be missed by a single PCR test. Of the other 80, five would have a false positive result of the PCR test. |
PCR, polymerase chain reaction; SSI, S. stercoralis infection. Estimates for sensitivity and specificity are here reported in %.
Studies included conventional PCR, nested PCR, real-time PCR
b Either Baermann method, agar plate culture, Harada-Mori culture, or a combination of fecal methods