| Literature DB >> 35573006 |
Ju Jiang1,2, Constanza Martínez-Valdebenito3, Thomas Weitzel4,5, Christina M Farris1, Gerardo Acosta-Jamett6,7, Katia Abarca3, Allen L Richards2,8.
Abstract
Scrub typhus is a potentially severe rickettsiosis, caused by Orientia tsutsugamushi in the Asia-Pacific region. Recently, however, two distinct pathogens, "Candidatus Orientia chuto" and "Candidatus Orientia chiloensis", have been discovered in the Middle East and South America, respectively. Since the novel pathogens differ significantly from O. tsutsugamushi, many established diagnostic methods are unreliable. This work describes the development and validation of a new quantitative real-time PCR (qPCR) assay (Orien16S) for the detection of all known Orientia species. Based on a 94 bp sequence of the 16S rRNA gene (rrs), Orien16S recognized DNA samples from O. tsutsugamushi (n = 41), Ca. O. chiloensis (n = 5), and Ca. O. chuto (n = 1), but was negative for DNA preparations from closely related rickettsiae and other members of the order Rickettsiales (n = 22) as well as unrelated bacterial species (n = 11). After its implementation in Chile, the assay was verified, correctly identifying all tested eschar and buffy coat samples (n = 28) of clinical suspected cases. Furthermore, Orien16S detected Orientia DNA in trombiculid mites collected in endemic regions in southern Chile. The presented novel qPCR assay provides a useful tool for detecting Orientia and diagnosing scrub typhus from all geographical regions.Entities:
Keywords: Candidatus Orientia chiloensis; Chile; Orien16S; Orientia; South America; molecular diagnostic techniques; quantitative real-time PCR (qPCR); scrub typhus
Year: 2022 PMID: 35573006 PMCID: PMC9095740 DOI: 10.3389/fmed.2022.831045
Source DB: PubMed Journal: Front Med (Lausanne) ISSN: 2296-858X
DNA preparations from bacterial strains and other sources included in the validation of the novel qPCR assay, Orien16S.
| New | Other Rickettsiales agents | Other bacteria and controls | ||
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| Karp (New Guinea) | Woods (Australia) |
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| Kato (Japan) | Sido (Australia) |
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| Gilliam (Burma) | BSR178 (New Zealand) |
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| AFC-3 (Thailand) | Buie (New Guinea) | |||
| AFC-30 (Thailand) | Calcutta (India) |
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| AFPL-12 (Thailand) | Ikeda (Japan) |
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| TA-678 (Thailand) | Kawasaki (South Korea) |
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| TA-686 (Thailand) | 18-032111 (Pakistan) |
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| TA-763 (Thailand) | 18-032460 (Malaysia) |
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| TH-1812 (Thailand) | 18-030642 (China) |
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| TH-1814 (Thailand) | MAK-110 (China-Taiwan) |
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| TH-1817 (Thailand) | MAK-119 (China-Taiwan) | Human DNA | ||
| CRF136 (Thailand) | MAK-243 (China-Taiwan) | Mouse DNA 1 | ||
| FPW1038 (Thailand) | TM1073 (Laos) |
| Mouse DNA 2 | |
| FPW2016 (Thailand) | TM1324 (Laos) | Mouse DNA 3 | ||
| UT76 (Thailand) | Faulkner (Vietnam) | Mouse DNA 4 | ||
| UT221 (Thailand) | Hicks (Vietnam) | |||
| UT661 (Thailand) | Middleton (Vietnam) | |||
| Brown (Australia) | Volner (Philippines) |
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| Citrano (Australia) |
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| Domrow (Australia) |
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| Garton (Australia) |
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FIGURE 1Alignment of the rrs sequence at primer and probe sites.
Comparison of the amplification characteristics (Ct values) of Orien16S and Otsu47 qPCR assays with samples of Orientia tsutsugamushi, Ca. Orientia chuto, and Ca. Orientia chiloensis.
| qPCR Ct | qPCR Ct values | ||||
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| Strain | Orien16S | Otsu47 | Strain | Orien16S | Otsu47 |
| 28.29 | 30.19 | 28.08 | 28.25 | ||
| 29.32 | 30.24 | 26.23 | 27.36 | ||
| 27.99 | 29.11 | 21.66 | 22.19 | ||
| 21.73 | 22.77 | 28.89 | 30.82 | ||
| 29.46 | 30.27 | 30.75 | 32.03 | ||
| 29.03 | 30.26 | 30.5 | 31.3 | ||
| 20.59 | 22.19 | 21.89 | 20.68 | ||
| 31.58 | 32.65 | 29.78 | 30.73 | ||
| 30.07 | 31.26 | 30.82 | 32.05 | ||
| 28.68 | 29.18 | 30.45 | 31.24 | ||
| 28.87 | 29.98 | 27.49 | 28.17 | ||
| 28.57 | 29.36 | 33.58 | 33.44 | ||
| 26.65 | 26.97 | 36.26 | 37.63 | ||
| 18.78 | 20.7 | 34.69 | 35.86 | ||
| 20.85 | 20.75 | 36.12 | 35.38 | ||
| 29.22 | 29.8 | 22.84 | 23.3 | ||
| 28.31 | 29.88 | 29.23 | 29.42 | ||
| 29.21 | 30.29 | 28.43 | 42.82 | ||
| 24.32 | 25.35 | 42.3 | Negative | ||
| 29.45 | 30.46 | 36.56 | Negative | ||
| 30.32 | 30.91 | 31.25 | Negative | ||
| 19.43 | 20.52 | 26.27 | Negative | ||
| 27.53 | 28.61 | 32.25 | Negative | ||
| 25.77 | 26.87 | pOrien6 | 28.67 | 28.68 | |
Amplification results (Ct values) of new Orien16S qPCR assay in specimens from human scrub typhus cases and mite pools from Chiloé Island.
| Clinical samples | ||||
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| No. | Patient sex/age (years) | Sample type | Orien16S Ct | References |
| 1 | Male/43 | Eschar | 31.76 | ( |
| 2 | Male/56 | Eschar | 24.65 | ( |
| 3 | Male/56 | Buffy coat | 35.62 | ( |
| 4 | Male/25 | Eschar | 29.76 | ( |
| 5 | Male/69 | Eschar | 25.65 | ( |
| 6 | Male/69 | Buffy coat | 29.77 | ( |
| 7 | Female/22 | Eschar | 27.38 | ( |
| 8 | Male/25 | Eschar | 28.09 | ( |
| 9 | Male/39 | Eschar | 28.76 | ( |
| 10 | Male/39 | Buffy coat | 26.8 | ( |
| 11 | Male/28 | Eschar | 31.58 | ( |
| 12 | Male/28 | Buffy coat | 32.85 | ( |
| 13 | Female/21 | Eschar | 25.99 | ( |
| 14 | Male/20 | Eschar | 29.41 | ( |
| 15 | Male/17 | Eschar | 35.54 | ( |
| 16 | Male/55 | Eschar | 34.16 | ( |
| 17 | Male/73 | Eschar | 30.97 | ( |
| 18 | Female/49 | Eschar | 27.12 | ( |
| 19 | Female/49 | Buffy coat | 35.12 | ( |
| 20 | Female/30 | Eschar | 24.35 | ( |
| 21 | Male/54 | Eschar | 25.12 | ( |
| 22 | Male/63 | Eschar | 26.28 | ( |
| 23 | Female/23 | Eschar | 28.4 | ( |
| 24 | Male/53 | Eschar | 23.45 | ( |
| 25 | Male/41 | Eschar | 24.55 | ( |
| 26 | Female/54 | Eschar | 26.82 | ( |
| 27 | Male/44 | Eschar | 29.39 | ( |
| 28 | Male/62 | Eschar | 29.23 | ( |
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| 1 | A olivacea/site4_1 | Mite pool | 33.48 | ( |
| 2 | A olivacea/site4_4 | Mite pool | 30.94 | ( |
| 3 | A sanborni/site4_1 | Mite pool | 33.14 | ( |
| 4 | A olivacea/site6_1 | Mite pool | 31.64 | ( |