Comparison between Aptima Assays (Hologic) and the Allplex STI Essential Assay (Seegene) for the diagnosis of Sexually transmitted infections

Authors: Adolfo de Salazar ^aff001; Beatriz Espadafor ^aff002; Ana Fuentes-López ^aff001; Antonio Barrientos-Durán ^aff001; Luis Salvador ^aff002; Marta Álvarez ^aff001; Federico García ^aff001
Authors place of work: Hospital Universitario San Cecilio, Servicio de Microbiología, Instituto de Investigación Ibs, Granada, Spain ^aff001; Hospital Universitario Virgen de las Nieves, Servicio de Dermatología, Centro de ETS, Granada, Spain ^aff002
Published in the journal: PLoS ONE 14(9)
Category: Research Article
doi: https://doi.org/10.1371/journal.pone.0222439

Summary

Sexually transmitted infections (STIs) remain a worldwide problem and a severe threat to public health. The purpose of this study was to compare Aptima^® Assays (Hologic^®) and the Allplex^™ STI Essential Assay (Seegene^®) for the simultaneous detection of Chlamydia trachomatis, Neisseria gonorrhoeae, Trichomonas vaginalis and Mycoplasma genitalium in clinical practice. The Aptima^® assays (Hologic^®) are based on a transcription-mediated amplification (TMA) method. The Allplex^™ STI Essential assay (Seegene^®) is based on a multiplex Real-Time PCR (RT-PCR) method. A total of 622 clinical samples from different anatomical sites were tested using both methods. A total of 88 (14.1%) and 66 (10.6%) positive samples were found for any of the TMA assays used and for the RT-PCR assay, respectively. Aptima^® assays showed a slightly higher rate of positive results for all pathogens except for T. vaginalis, the results of which were similar to those obtained with Allplex^™. The most commonly detected pathogen was C. trachomatis (37 samples; 5.9% using TMA assays) and the anatomical site with the highest prevalence of microorganisms was a non-urogenital site, the pharynx (27 positive samples; 4.3%). Using the Aptima^® assays as reference method, the comparison showed that the average specificity of multiplex RT-PCR was 100.0% for the four pathogens. However an average sensitivity of 74.5% was observed, showing 95.2% (CI95%; 93.6–96.9) of overall concordance (κ = 0.80). In conclusion, the Aptima^® assays show a higher sensitivity on a wide range of sample types compared to the Allplex^™ assay.

Keywords:

Biology and life sciences – Biochemistry – Nucleic acids – Organisms – Eukaryota – Research and analysis methods – Molecular biology – Molecular biology techniques – Anatomy – Medicine and health sciences – Microbiology – Medical microbiology – Microbial pathogens – Bacterial pathogens – Bacteria – Pathology and laboratory medicine – Pathogens – Physiology – infectious diseases – Body fluids – Artificial gene amplification and extension – Polymerase chain reaction – Sexually transmitted diseases – Reverse transcriptase-polymerase chain reaction – Urine – Chlamydia – Neisseria – Protists – Trichomonas – Trichomonas vaginalis – Chlamydia trachomatis – Neisseria gonorrhoeae – Chlamydia infection

Introduction

Sexually transmitted infections (STIs) remain a worldwide problem and a severe threat to public health. In 2012, approximately 130.9, 78.3, and 142.6 million new cases of Chlamydia trachomatis, Neisseria gonorrhoeae, and Trichomonas vaginalis infections, respectively, were estimated globally [1]. For Mycoplasma genitalium, prevalence has been estimated at 1.3% in high-income countries and 3.9% in low-income countries [2]. These microorganisms are responsible for a variety of clinical syndromes in women and men, such as urethritis, cervicitis, prostatitis and vaginitis [3–6], which may lead to severe complications and long-term sequelae, including pelvic inflammatory disease, infertility, chronic pelvic pain, ectopic pregnancy, neurological and cardiovascular disease in adults, premature delivery, neonatal death, severe disability or blindness in infants, and increased risk of HIV acquisition and transmission [7, 8].

Prompt recognition and appropriate treatment are essential for the control of transmission of STIs, and this requires sensitive and accurate laboratory diagnostic methods. The implementation of nucleic acid amplification tests (NAATs) has revolutionized diagnostics in the detection of C. trachomatis, N. gonorrhoeae, T. vaginalis and M. genitalium, due to their numerous advantages over conventional methods [9]. However, these tests traditionally required separate processes for nucleic acid extraction and amplification/detection, which may increase the risk of errors (manipulation errors, contamination during the extraction step, etc.), especially in high-volume diagnostic laboratories. Another limitation is the need for batch samples, which may delay diagnosis and treatment initiation.

The use of multiplex RT-PCR for the diagnosis of STI is widespread in Microbiology laboratories, because they offer a large panel of microorganisms in a simple reaction, at a low cost. However, these techniques may have a lower sensitivity than others commercially available.

Currently there are assays for the diagnosis of STI based on transcription-mediated amplification (TMA) targeting directly ribosomal RNA (rRNA), with the advantage of a higher number of copies per cell compared to DNA-based tests, which only target one copy. Assays based on TMA potentially increase sensitivity of detection compared to assays based on RT-PCR targeting single-copy genes [10–15]. To date, only a few studies compare these two methodologies for the simultaneous diagnosis of the 4 most important pathogens causing STIs [16, 17].

The objective of this study was to assess the performance of multiplex RT-PCR [Allplex^™ STI Essential (Seegene^®, Seoul, South Korea)]. This is an in vitro diagnostic (IVD) and CE-marked system for the simultaneous detection of C. trachomatis, N. gonorrhoeae, T. vaginalis and M. genitalium. The following FDA-cleared assays based on TMA were used as the reference method: Aptima Combo 2^® (for C. trachomatis and N. gonorrhoea), Aptima^® T. vaginalis and Aptima^® M. genitalium (Hologic^®, San Diego, USA)].

Material and methods

Patients

The study was conducted between May 2017 and November 2017 in Granada, Spain. A total of 375 patients from the Centre for Sexually Transmitted Diseases in Granada were enrolled in the study. The median age of males (n = 243; 65%) and females (n = 132; 35%) was 29 years [IQR: 23–37]. The study was designed and conducted according to the principles expressed in the Declaration of Helsinki and it was approved by the local Ethics Committee of Hospital Universitario San Cecilio. Verbal informed consent was obtained from all participants.

Data underlying the findings described in this study have been deposited to Figshare and they are accessible via https://doi.org/10.6084/m9.figshare.9159746.v2. All other relevant data are shown in the present manuscript.

Specimen collection

A total of 622 prospective clinical specimens from different anatomical sites (urine and endocervical, pharyngeal and anal swabs) according to the reported type of sexual practices (vaginal, oral and/or anal intercourse) of 375 participants were collected in duplicate. Table 1 shows a detailed description of the anatomical location of the collected samples. Specimens for routine testing were collected with dry swabs. The swabs were suspended in 2 mL of 1X Phosphate Buffered Saline solution (PBS) as transport system. Urine samples for TMA-assay testing were collected using the Aptima^® Urine Collection Kit for Male and Female Specimens (Hologic, San Diego, USA). Female endocervical and male urethral samples were collected with the Aptima^® Unisex Swab Specimen collection kit (Hologic, San Diego, USA). The Aptima^® Multitest Swab Specimen Collection Kit (Hologic, San Diego, USA) was used for the collection of pharyngeal and anal specimens. Random sampling was performed by alternating the collection of specimens for routine testing and specimens for Aptima^® testing. The distribution of the types of clinical specimens (622) was the following: 218 (35%) pharyngeal swabs, 214 (35%) first-void urine samples, 107 (17%) endocervical swabs and 83 (13%) rectal swabs. After collection, specimens were stored at 4°C until testing, generally, for two or three days after specimen collection. All NAATs were performed in parallel by the same technician.

<h2>Distribution of the collected samples.</h2> — Tab. 1.
Distribution of the collected samples.

Real-Time multiplex PCR assay

Testing was performed using the multiplex RT-PCR Allplex^™ STI Essential Assay (Seegene, Seoul, Korea). This assay can simultaneously detect 7 STI pathogens (C. trachomatis, N. gonorrhoeae, T. vaginalis, M. genitalium, M. hominis, U. urealyticum and U. parvum) in a single tube by using dual priming oligonucleotide (DPO^™) and multiple detection temperatures (MuDT^™) technologies, providing individual C_t values for multiple pathogens in a single channel. The DPO system differs structurally and functionally from the conventional primer system by including a poly deoxyinosine (I) linker, between two segments of primer sequences. This poly (I) linker allows dividing the DPO primer into two perfectly functional segments with different hybridization temperatures [18]. The elongation will be conducted when the two segments hybridize correctly giving rise to a high specificity between similar or related sequences. Previous nucleic acid extraction was performed (400 μL sample volume) using MagNA Pure 96 System (Roche); nucleic acids were eluted in 50 μL (final volume). Real-time PCR was performed in a CFX-96 real-time thermocycler (Bio-Rad, CA, USA), according to the manufacturer’s instructions. To maximize cost-efficiency without a significant delay in reporting, routine testing was performed in batches every Tuesday and Friday. For this study, only the results for C. trachomatis, N. gonorrhoeae, T. vaginalis and M. genitalium were analyzed.

Transcription-mediated amplification assay

The Aptima^® assays comprise three main steps: target capture, TMA of the species-specific targets in the rRNA, and target detection by hybridization with complementary probes linked to chemiluminescent labels. The TMA step consists of a target nucleic acid amplification method using RNA transcription (RNA polymerase) and DNA synthesis (reverse transcriptase) to produce a RNA amplicon from a target nucleic acid; TMA can be used to target both RNA and DNA [19].

Aptima^® M. genitalium (MG), Aptima^® Combo 2 (detecting both C. trachomatis, N. gonorrhoeae in one sample) and Aptima^® T. vaginalis assays were used on the Panther^® system (Hologic, San Diego). This system is a fully automated testing platform with true sample-to-result automation allowing sample testing with Aptima^® assays, therefore avoiding the separate DNA extraction step. For this evaluation, samples collected for the Aptima^® assays were stored at 4°C and run on the same day as the RT-PCR.

Data analysis

Sensitivity (SE), specificity (SP) and kappa coefficient (κ) of the multiplex RT-PCR were calculated and compared with TMA assays for detection of C. trachomatis, N. gonorrhoeae, M. genitalium and T. vaginalis using the statistical package SPSS, version 23 (IBM, Chicago, IL, USA). The corresponding two-tailed 95% score (Wilson) confidence intervals (CIs) were also estimated.

Results

A total of 622 samples were tested using both methods. Positive results were found in 88 (14.1%) out of 622 samples for all the Aptima^® assays used. Regarding the Allplex^™ assay, only 66 (10.6%) out of 622 samples showed positive results. Table 2 and S1 Table show the diagnostic performance of the systems used for detection of the different pathogens. The TMA-based assays performed on the Panther^® platform showed slightly higher positive results for C. trachomatis, N. gonorrhoeae and M. genitalium, while results for the T. vaginalis samples were similar for both RT-PCR (Allplex^™) and TMA (Aptima^®) assays. The most frequently detected pathogen was C. trachomatis (37 samples; 5.9%).

<h2>Diagnostic performance of Allplex<sup>™</sup> STI Essential assays in relation to the Aptima<sup>®</sup> assays for <i>C</i>. <i>trachomatis</i>, <i>N</i>. <i>gonorrhoeae</i>, <i>M</i>. <i>genitalium</i> and <i>T</i>. <i>vaginalis</i>.</h2> — Tab. 2.
Diagnostic performance of Allplex^™ STI Essential assays in relation to the Aptima^® assays for C. *trachomatis*, N. *gonorrhoeae*, M. *genitalium* and T. *vaginalis*.

The TMA-positive samples were further analyzed according to their anatomical site. Results revealed that a non-urogenital sample, the pharynx, was the most frequent site with a positive result (29 positive samples; 4.7%) followed by urine (27 positive samples; 4.3%), endocervical (22 positive samples; 3.5%) and anal samples (17 positive samples; 2.7%) (Tables 3 and 4). A total of 14 more samples were found positive for M. genitalium using Aptima^® assays (n = 24) than positive samples for M. genitalium identified using the Allplex^™ STI Essential assay (n = 10); ten of these Aptima-positive samples were collected from pharyngeal swabs.

<h2>Anatomical distribution and prevalence of the Aptima<sup>®</sup>-positive samples.</h2> — Tab. 3.
Anatomical distribution and prevalence of the Aptima^®-positive samples.

<h2>Anatomical distribution and prevalence of the Allplex<sup>™</sup>-positive samples.</h2> — Tab. 4.
Anatomical distribution and prevalence of the Allplex^™-positive samples.

The diagnostic performance of the Allplex assay was evaluated by the calculation of SE and SP parameters. Concordance between the Aptima^® and the Allplex assays was determined through the calculation of the Cohen’s Kappa index, κ coefficient of the Allplex assay in relation to the Aptima^® assays (reference method) for the detection of C. trachomatis, N. gonorrhoeae, M. genitalium and T. vaginalis (Table 2). A specificity of 100.0% was found for the four pathogens, however an average sensitivity of 74.5% was observed for the Allplex assay. Both methods (TMA and multiplex RT-PCR) have shown a variable consistency depending on the microorganism detected, with κ values ranging between 0.58 for M. genitalium and 0.91 for C. trachomatis. In general, a concordance of 95.2% (CI95%; 93.6–96.9) and κ = 0.80 were obtained between both methods. Among the 622 samples, there were 28 discrepancies: 4 anal, 3 endocervical, 13 pharyngeal and 8 urine samples. Co-infections were observed in 7 samples from 7 different patients and inconsistent results were detected in 6 of these patients. A detailed description of these results is shown in Table 5.

<h2>Discordant results between Aptima<sup>®</sup> and Allplex<sup>™</sup> assays regarding the detection of <i>C</i>. <i>trachomatis</i>, <i>M</i>. <i>genitalium and N</i>. <i>gonorrhoeae</i>.</h2> — Tab. 5.
Discordant results between Aptima^® and Allplex^™ assays regarding the detection of C. *trachomatis*, M. *genitalium and N*. *gonorrhoeae*.

Discussion

The relatively high prevalence of STIs and the need for a rapid and accurate diagnostic tool for their detection justifies that any new methodology must be thoroughly evaluated before its implementation in routine laboratory practice. In this study, we evaluated the performance of TMA-based assays (Aptima Combo 2^® (for C. trachomatis and N. gonorrhoea), Aptima^® T. vaginalis and Aptima^® M. genitalium) on the Panther^® platform for simultaneous detection of C. trachomatis, N. gonorrhoeae, T. vaginalis and M. genitalium in comparison with a multiplex RT-PCR assay (Allplex^™ STI Essential, Seegene^®). Although Aptima^® assays have previously shown good performances in the diagnosis of these pathogens [10–15], this is, to our knowledge, the first time that the detection of these four pathogens together has been compared to Allplex^™ STI Essential RT-PCR-based assay. The effectiveness of the Allplex^™ assay has also been previously proven [20–22].

Both systems showed the highest prevalence of C. trachomatis in the analyzed samples, which is in line with this pathogen being the most frequently reported STI in Europe [23]. The sensitivity of the TMA assays was higher for most pathogens compared to multiplex RT-PCR. It is very remarkable that most of the samples responsible for this higher sensitivity were pharyngeal swab samples, and that M. genitalium was more frequently detected in this location with TMA assays. For most bacterial STI, the throat is the anatomical location with the lowest number of positive samples [24] however our findings at least in the case of M. genitalium, confirm the results of recent reports in the literature [25]. Our results confirm that other sites should always be considered based on patient’s sexual habits [26]. In fact, using urogenital samples alone overlooks many infections, resulting in many patients failing to receive proper treatment [27].

The sensitivity and specificity of these TMA assays have been evaluated previously, with sensitivities and specificities > 90% [13, 14, 28], however recently, false-negative Chlamydia trachomatis have been reported using Aptima Combo2^® assays in Finland and Sweden due to a 23S rRNA C1515T mutation [29, 30]. It is important to mention that a single genetic target region should not be trusted in molecular diagnosis of infections to avoid underdiagnosis of possible mutants, this could be a limitation of this assay, that only amplify chlamydial 23S rRNA.

Our study has two important limitations. First, we could not resolve all discordant results with a third test because our sample volume was low and we did not want to dilute the sample to prevent losing sensitivity. Thereof, we could not calculate the positive predictive value and negative predictive value of this test, and we could not rule out that the higher sensitivity of the TMA assays could be due to false positive detections. Second, T. vaginalis specimens found in pharyngeal swabs with the RT-PCR test were not included in the final analysis. In fact, we found 19 pharyngeal samples that were scored positive for T. vaginalis only with the Allplex^™ test; it is well documented that DNA-based methods may lack specificity for discriminating T. vaginalis from some other oral Trichomonas species existing in the pharyngeal microbiota, such as Trichomonas tenax [31, 32].

Our results confirm the effectiveness of the Aptima^® assays for STI diagnosis, providing additional evidence supporting the implementation of this methodology for routine testing in clinical diagnostics. Importantly, this TMA technology provides important features for laboratory automation and daily clinical practice. Thus, patients might benefit highly from this technology, as they can be evaluated and diagnosed at the same medical visit.

Supporting information

S1 Table [docx]
Details regarding the number of positive and negative samples identified with Aptima and Allplex assays.

Zdroje

1. World Health Organization. Report on global sexually transmitted infection surveillance 2015. WHO; 2016. https://apps.who.int/iris/handle/10665/249553

2. Baumann L, Cina M, Egli-Gany D, Goutaki M, Halbeisen FS, Lohrer G-R, et al. Prevalence of Mycoplasma genitalium in different population groups: systematic review andmeta-analysis. Sex Transm Infect. 2018;94(4):255–62. doi: 10.1136/sextrans-2017-053384 29440466

3. Manhart LE, Broad JM, Golden MR. Mycoplasma genitalium: Should We Treat and How? Clin Infect Dis. 2011;53(suppl_3):S129–42.

4. Malhotra M, Sood S, Mukherjee A, Muralidhar S, Bala M. Genital Chlamydia trachomatis: An update. Indian J Med Res. 2013;138(3):303–16. 24135174

5. Alirol E, Wi TE, Bala M, Bazzo ML, Chen X-S, Deal C, et al. Multidrug-resistant gonorrhea: A research and development roadmap to discover new medicines. PLOS Medicine. 2017;14(7):e1002366. doi: 10.1371/journal.pmed.1002366 28746372

6. Edwards T, Burke P, Smalley H, Hobbs G. Trichomonas vaginalis: Clinical relevance, pathogenicity and diagnosis. Crit Rev Microbiol. 2014;1–12.

7. Vos T, Barber RM, Bell B, Bertozzi-Villa A, Biryukov S, Bolliger I, et al. Global, regional, and national incidence, prevalence, and years lived with disability for 301 acute and chronic diseases and injuries in 188 countries, 1990–2013: a systematic analysis for the Global Burden of Disease Study 2013. The Lancet. 2015;386(9995):743–800.

8. Sieving RE, Gewirtz O’Brien JR, Saftner MA, Argo TA. Sexually transmitted diseases among us adolescents and young adults. Nursing Clinics of North America. 2019;54(2):207–25. doi: 10.1016/j.cnur.2019.02.002 31027662

9. Nye MB, Schwebke JR, Body BA. Comparison of APTIMA Trichomonas vaginalis transcription-mediated amplification to wet mount microscopy, culture, and polymerase chain reaction for diagnosis of trichomoniasis in men and women. Am J Obstet Gynecol. 2009;200(2):188.e1–188.e7.

10. Boyadzhyan B, Yashina T, Yatabe JH, Patnaik M, Hill CS. Comparison of the APTIMA CT and GC Assays with the APTIMA Combo 2 Assay, the Abbott LCx Assay, and Direct Fluorescent-Antibody and Culture Assays for Detection of Chlamydia trachomatis and Neisseria gonorrhoeae. J Clin Microbiol. 2004;42(7):3089–93. doi: 10.1128/JCM.42.7.3089-3093.2004 15243065

11. Golparian D, Tabrizi SN, Unemo M. Analytical Specificity and Sensitivity of the APTIMA Combo 2 and APTIMA GC Assays for Detection of Commensal Neisseria Species and Neisseria gonorrhoeae on the Gen-Probe Panther Instrument: Sex Transm Dis. 2013;40(2):175–8. doi: 10.1097/OLQ.0b013e3182787e45 23324980

12. Wroblewski JKH, Manhart LE, Dickey KA, Hudspeth MK, Totten PA. Comparison of transcription-mediated amplification and PCR assay results for various genital specimen types for detection of Mycoplasma genitalium. J Clin Microbiol. 2006;44(9):3306–12. doi: 10.1128/JCM.00553-06 16954265

13. Tabrizi SN, Unemo M, Limnios AE, Hogan TR, Hjelmevoll S-O, Garland SM, et al. Evaluation of Six Commercial Nucleic Acid Amplification Tests for Detection of Neisseria gonorrhoeae and Other Neisseria Species. J Clin Microbiol. 2011;49(10):3610–5. doi: 10.1128/JCM.01217-11 21813721

14. Chernesky M, Jang D, Luinstra K, Chong S, Smieja M, Cai W, et al. High Analytical Sensitivity and Low Rates of Inhibition May Contribute to Detection of Chlamydia trachomatis in Significantly More Women by the APTIMA Combo 2 Assay. J Clin Microbiol. 2006;44(2):400–5. doi: 10.1128/JCM.44.2.400-405.2006 16455891

15. Hokynar K, Hiltunen-Back E, Mannonen L, Puolakkainen M. Prevalence of Mycoplasma genitalium and mutations associated with macrolide and fluoroquinolone resistance in Finland. Int J STD AIDS. 2018;29(9):904–7. doi: 10.1177/0956462418764482 29631509

16. Rumyantseva T, Golparian D, Nilsson CS, Johansson E, Falk M, Fredlund H, et al. Evaluation of the new AmpliSens multiplex real-time PCR assay for simultaneous detection of Neisseria gonorrhoeae, Chlamydia trachomatis, Mycoplasma genitalium, and Trichomonas vaginalis. APMIS. 2015;123(10):879–86. doi: 10.1111/apm.12430

17. Levett PN, Brandt K, Olenius K, Brown C, Mont- gomery K, Horsman GB. Evaluation of three automated nucleic acid amplification systems for detection of Chlamydia trachomatis and Neisseria gonorrhoeae in first-void urine specimens. J Clin Microbiol 2008;46:2109–11. doi: 10.1128/JCM.00043-08 18400919

18. Chun J-Y, Kim K-J, Hwang I-T, Kim Y-J, Lee D-H, Lee I-K, et al. Dual priming oligonucleotide system for the multiplex detection of respiratory viruses and SNP genotyping of CYP2C19 gene. Nucleic Acids Res. 2007;35(6):e40. doi: 10.1093/nar/gkm051 17287288

19. Gonzales F, McDonough SH. Application of transcription-mediated amplification to quantification of gene sequences. In: Ferré F. (eds). Gene Quantification. Advanced Biomedical Technologies. Birkhäuser Boston; 1998. p. 189–201. http://link.springer.com/10.1007/978-1-4612-4164-5_11

20. Choe H-S, Lee DS, Lee S-J, Hong S-H, Park DC, Lee M-K, et al. Performance of Anyplex™ II multiplex real-time PCR for the diagnosis of seven sexually transmitted infections: comparison with currently available methods. Int J Infect Dis. 2013;17(12):e1134–40. doi: 10.1016/j.ijid.2013.07.011

21. Del Prete R, Ronga L, Lestingi M, Addati G, Angelotti UF, Di Carlo D, et al. Simultaneous detection and identification of STI pathogens by multiplex Real-Time PCR in genital tract specimens in a selected area of Apulia, a region of Southern Italy. Infection. 2017;45(4):469–77. doi: 10.1007/s15010-017-1002-7 28260146

22. Robinet S, Parisot F. Accreditation of a multiplex real time PCR assay for detection and semi-quantitative determination of pathogens responsible of sexually-transmitted infections. Ann Biol Clin (Paris). 20187–8;(4):459–476.

23. European Centre for Disease Prevention and Control. Chlamydia infection. In: ECDC. Annual epidemiological report for 2017. Stockholm: ECDC; 2019. http://ecdc.europa.eu/sites/portal/files/documents/AER_for_2017-chlamydia-infection.pdf

24. Hananta IPY, de Vries HJC, van Dam AP, van Rooijen MS, Soebono H, Schim van der Loeff MF. Spontaneous clearance of pharyngeal gonococcal infections: a retrospective study in patients of the sexually transmitted infections clinic, Amsterdam, the Netherlands 2012–2015. Sexually Transmitted Diseases. 2018;1.

25. Le Roy C, Pereyre S, Hénin N, Bébéar C. French Prospective Clinical Evaluation of the Aptima Mycoplasma genitalium CE-IVD Assay and Macrolide Resistance Detection Using Three Distinct Assays. Munson E, editor. J Clin Microbiol. 2017;55(11):3194–200. doi: 10.1128/JCM.00579-17 28794183

26. Whittles LK, Didelot X, Grad YH, White PJ. Testing for gonorrhoea should routinely include the pharynx. Lancet Infect Dis. 2018;18(7):716–7.

27. Garner AL, Schembri G, Cullen T, Lee V. Should we screen heterosexuals for extra-genital chlamydial and gonococcal infections? Int J STD AIDS. 2015;26(7):462–6. doi: 10.1177/0956462414543120 25013220

28. Cheng A, Kirby JE. Evaluation of the Hologic Gen-Probe PANTHER, APTIMA Combo 2 Assay in a Tertiary Care Teaching Hospital. Am J Clin Pathol. 2014;141(3):397–403. doi: 10.1309/AJCPFQ25SQVZAWHZ 24515768

29. Rantakokko-Jalava K, Hokynar K, Hieta N, Keskitalo A, Jokela P, Muotiala A, et al. Chlamydia trachomatis samples testing falsely negative in the Aptima Combo 2 test in Finland, 2019. Eurosurveillance. 2019;24(22):1900298.

30. Unemo M, Hansen M, Hadad R, Lindroth Y, Fredlund H, Puolakkainen M, et al. Finnish new variant of Chlamydia trachomatis escaping detection in the Aptima Combo 2 assay also present in Örebro County, Sweden, May 2019. Eurosurveillance. 2019;24(26):1900370.

31. Chapin K, Andrea S. APTIMA® Trichomonas vaginalis, a transcription-mediated amplification assay for detection of Trichomonas vaginalis in urogenital specimens. Expert Review of Molecular Diagnostics. 2011;11(7):679–88. doi: 10.1586/erm.11.53

32. Kucknoor AS, Mundodi V, Alderete J. Genetic identity and differential gene expression between Trichomonas vaginalis and Trichomonas tenax. BMC Microbiol. 2009;9(1):58.

Comparison between Aptima Assays (Hologic) and the Allplex STI Essential Assay (Seegene) for the diagnosis of Sexually transmitted infections

Summary

Keywords:

Introduction

Material and methods

Patients

Specimen collection

Distribution of the collected samples.

Real-Time multiplex PCR assay

Transcription-mediated amplification assay

Data analysis

Results

Diagnostic performance of Allplex™ STI Essential assays in relation to the Aptima® assays for C. trachomatis, N. gonorrhoeae, M. genitalium and T. vaginalis.

Anatomical distribution and prevalence of the Aptima®-positive samples.

Anatomical distribution and prevalence of the Allplex™-positive samples.

Discordant results between Aptima® and Allplex™ assays regarding the detection of C. trachomatis, M. genitalium and N. gonorrhoeae.

Discussion

Supporting information

Zdroje

PLOS One

Získaná hemofilie - Povědomí o nemoci a její diagnostika

Eozinofilní granulomatóza s polyangiitidou

Diagnostic performance of Allplex^™ STI Essential assays in relation to the Aptima^® assays for C. trachomatis, N. gonorrhoeae, M. genitalium and T. vaginalis.

Anatomical distribution and prevalence of the Aptima^®-positive samples.

Anatomical distribution and prevalence of the Allplex^™-positive samples.

Discordant results between Aptima^® and Allplex^™ assays regarding the detection of C. trachomatis, M. genitalium and N. gonorrhoeae.