DOI: https://doi.org/10.21203/rs.2.24375/v1
Background: Trichomoniasis resulting from Trichomonas vaginalis (T. vaginalis) has been considered as a commonly seen disease with the transmission way of sex. At present, the detection methods of T. vaginalis mainly include wet mount microscopy, culture, PCR, immunofluorescence and ELISA. However, all of these detection methods exist shortcomings.
Methods: In this study, a loop-mediated isothermal amplification (LAMP) assay that targeted the species-specific sequence of adhesion protein 65 (AP65) gene had been conducted to detect T. vaginalis. The optimum reaction system and conditions were optimized in this rapid detection method.
Results: The results of sensitivity analysis showed that the LAMP assay targeting the AP65 gene was 1000 times more sensitive than the nested PCR targeting the actin gene commonly used for detection of T. vaginalis, and the detecting limitation of the former was 10 trichomonad. Moreover, the amplification of the target gene AP65 by LAMP assay exhibited high specificity and the product was exclusively from T. vaginalis. The detection technique of LAMP did not exhibit cross-reactivity with the common pathogens of Trichinella spiralis, Toxoplasma gondii, Escherichia coli, Candida albicans, Staphylococcus aureus, Haemophilus.
Conclusions: According to the present study, the LAMP assay with the target of AP65 gene, was suitable for the early diagnosis of T. vaginalis infections. Consequently, the LAMP assay was proposed by the current study as a point-of-care examination and an alternative molecular tool which exhibited the potential value in the treatment, control and prevention of trichomoniasis transmission and relevant complication.
Trichomoniasis, which is resulting from T. vaginalis, a kind of protozoa with flagella, has been considered as a commonly seen curable disease with the transmission approach of sex and the quantity of affected people all around the world reaches 276.4 million [1, 2]. T. vaginalis is parasitized in the vagina and urethra of female, and in the urethra and prostate gland of male [3, 4]. The disease is characterized by asymptomatic status with the pathogen and acute or chronic inflammation [5]. As an extracellular parasite, T. vaginalis adheres to the surface of epithelial cells, and the damage to epithelial cells mainly depends on direct contact [6]. The wound of the parasitic site of epithelial cells was caused by the mechanical action of pleomorphic pseudopodia of trophozoite passing through and wrapping and flagellum movement, the digestion of releasing hydrolase, phagocytosis, and complex effects of exfoliative factors, after T. vaginalis infected human reproductive urinary tract. Then inflammation of tissues and organs was caused [7, 8].
According to statistics, more than 170 million people were infected with the disease every year in the world, and the infection rate of people around the world was different and had an increasing trend [9]. In the United States, nearly 5 million people were infected with T. vaginalis every year, while the infection rate was 24.3% in Japan, 23.8% in Uganda and 18.0% in South Africa [10]. In China, the infection rate in different places and people fluctuated greatly, ranging from a few percent to dozens of percent [11-13]. Clinical manifestations of the disease in women possibly contain vulvovaginal irritation, lower abdominal pain, dyspareunia, dysuria, malodorous vaginal discharge [2, 14], although the infection is usually asymptomatic in men or in a few cases with the clinical manifestations of dysuria, irritation, urethral discharge [15, 16]. In addition, pregnant women infected with T. vaginalis could cause decrease of birth weights, premature rupture of fetal membrane, premature delivery, abortion [17]. Recent studies have shown that T. vaginalis infection is also related to cervical cancer in women [18], prostate cancer in men and infertility [18, 19]. The widespread infection and prevalence of T. vaginalis increased the risk of human infection with human immunodeficiency virus (HIV) and mycoplasma, and T. vaginalis has become an important co-factor of HIV infection [20].
The accurate diagnosis of trichomoniasis is an important link in the prevention and treatment of the disease, and it is of great significance to prevent the transmission of the disease. At present, the detection methods of T. vaginalis mainly contain wet mount microscopy, PCR, culture, immunofluorescence as well as ELISA [21, 22]. Among the diagnostic methods, the wet mount microscopy is low in cost, but poor in sensitivity [23]. The method of culture T. vaginalis is widely recognized as the "gold standard" for diagnosing trichomoniasis [24]. The sensitivity of the diagnostic method is high, but it takes a long time and requires high quality specimens, and microscopic examiner needs to be professional and experienced. PCR detection is highly sensitive and specific, but it relies on the expensive instrument, and the amplified products need to be analyzed by gel electrophoresis [25]. The fluor immunofluorescence and ELISA are sensitive, but the specificity is poor, and the cost of antibody is expensive, and the detection time is long [26]. In 2000, Notomi et al. established LAMP technology, which had the advantages of simplicity, rapidity, high sensitivity, strong specificity and low cost [27]. The technology could amplify a large number of target genes in a short time and isothermal condition. In addition, this technology has been applied to the detection of bacteria, viruses and other pathogens [28].
AP65, as a specific protein of T. vaginalis, is a dominant functional protein which is targeted both to the surface and hydrogenosomes, and mediate binding to host cells [29, 30]. Garcia et al indicated that TvAP65 was a prominent adhered protein of trichomonad compared to other adhesin, and the protein was the hydrogenosomal NAD-dependent decarboxylating malic enzyme [31]. In this study, we developed a novel way to detect T. vaginalis based on loop-mediated isothermal amplification targeting adhesion protein 65.
Parasites
In the current work, the strain of T. vaginalis was isolated from the vaginal secretions of female patients clinically exhibiting certain trichomoniasis symptoms in the Third Affiliated Hospital of Xinxiang Medical University. The culture of T. vaginalis was performed using 10% calf serum, TYM medium added with antibiotics (100 mg/ml ceftriaxone, 50 mg/ml ciprofloxacin), fungicides (2.5 mg/ml amphotericin B) in a humidified chamber containing 5% CO2 at 37 ℃. The stationary phase parasites (2 × 106 parasites) were collected using a centrifuge and used subsequently in the experiments.
DNA extraction of T. vaginalis
PBS (pH 7.2) was used to wash the T. vaginalis trophozoite for thrice, which was subsequently isolated by centrifugation under the velocity of 5000 rpm for five minutes and subjected to DNA extraction using commercial kits (OMEGA) in accordance with the instruction.
The DNA simple of Trichinella spiralis, Toxoplasma gondii, Escherichia coli, Candida albicans, Staphylococcus aureus, Haemophilus were stored in Xinxiang Key Laboratory of Pathogenic Biology.
Detection of actin gene from T. vaginalis using nest-PCR
DNA extracts were subjected to species-specific nested PCR for T. vaginalis actin (GenBank Accession No. AF237734). Briefly, the primary PCR was performed in a 25 μL reaction mixture consisting of 12.5 μL of 2×PCR Master Mix (YIFEI XUE BIOTECHNOLOGY, Nanjing, China), 1 μL (0.1 μmol/L) each of the primers OUT-F and OUT-R (Table 1), 1.0 μL of DNA template (100-200ng), and 9.5 μL of double distilled water. The procedures and conditions of amplifying DNA included: three minutes at 95 ℃ for denaturation, 95 ℃ for 45 s, 55 ℃ for 30 s, and 72 °C for 1 min through 35 cycles, and 72 ℃ for 10 minutes for final extension. Then the second PCR was performed as the primary PCR, and the products of primary PCR and IN-F and IN-R (Table 1) were used as template and primers in this reaction. Electrophoresis using 1.5% agarose stained by 1.0 μL of Goldview Safe DNA Gel Stain (Yifei Xue Biotechnology, Nanjing, China) in advance was used to resolve the obtained DNA sequences at 100 V and a UV transilluminator (UVP, Upland, CA, USA) was used to visualize the bands.
Designing the primers of LAMP
LAMP Designer version 1.02 (Premier Biosoft, Palo Alto, CA, USA) was used to design the specific LAMP primers of T. vaginalisAP65 on the basis of the sequence in NCBI (GenBank Accession No. U35243.1). Four primers including outer primers (AP65-F3, AP65-B3), inner and forward primers (AP65-BIP, AP65-FIP) were chosen (Table 1). BLAST search was used to assess the specificity of these primers towards the sequences of target genes recorded by NCBI (http://www.blast.ncbi.nlm.nih.gov).
Detection of AP65 gene of T. vaginalis by LAMP assays
The mixed reaction solution with the volume of 20 μL which contained Betaine (5M) 6 μL (Sigma, St. Louis, MO, USA), 10×Bst DNA polymerase Buffer 2 μL, dNTPs Mixture (10mM each) 2 μL, each of AP65-FIP and AP65-BIP (16μM) 1 μL, each of F3 and B3 (4μM) 1 μL, MgCl2 (25mM) 3 μL, 8.0 U Bst DNA polymerase (TaKaRa, Dalian, China) 1.5 μL, and ddH2O 1.5 μL was used to perform the LAMP assays. The temperature condition of the LAMP reaction system was 63 ℃ for 120 minutes during the incubation and 80 ℃ for 10 minutes during the termination in a heating block. The experiment contained negative control (ddH2O) and positive control (T. vaginalis DNA).
The LAMP products were assessed by gel electrophoresis and addition of SYBR GreenⅠ(Solarbio, Beijing, China). For gel electrophoresis, 1.5% agarose gel was used to resolve 5.0 μL of the product of LAMP, as mentioned in Section 2.4, and the positive result was indicated by the pattern of bands like ladders. For addition of SYBR GreenⅠ, 2.0 μL of 1000× SYBR GreenⅠwas added to the remainder 15 μL of LAMP products, and the positive result was revealed by dull to fluorescent signal or change of colors from orange to green under visible light.
Analytical sensitivity of detection of AP65 gene of T. vaginalis by LAMP assay
The DNA with the initial concentration of 90 ng/μL in 2.3 was diluted by 101 -1012 times and kept for use. The trophozoites of T. vaginalis were diluted to 103, 102, 101 and 1 respectively, and the DNA of these diluted samples was extracted. Then, the prepared DNA samples were amplified by nested PCR and LAMP respectively, as described above. All the experiments were conducted in triplicate independently.
Analytical specificity of detection of AP65 gene of T. vaginalis by LAMP assay
The examination of the analytical specificity of AP65 gene of T. vaginalis by LAMP assay was conducted for determining the cross-reactive degree among DNA extraction samples from various trichomonads, Trichinella spiralis, Toxoplasma gondii, Escherichia coli, Candida albicans, Staphylococcus aureus and Haemophilus with close relation. The experiment contained negative control (ddH2O) and positive control (T. vaginalis DNA). All the experiments were conducted in triplicate independently.
Detecting T. vaginalis by nested PCR and LAMP
T. vaginalis actin gene was amplified using nest PCR with specific primers, and a positive sequence of 1100 bp was obtained in line with the expectation (Fig.1A). There were no target amplicons in negative controls.
According to the results of electrophoresis, the products amplified by LAMP with the target of AP65 in T. vaginalis exhibited distinctive pattern of multiple bands (Fig.1B). An orange-to-green color change was observed under natural light or a dull to fluorescent signal under UV transilluminator, after addition of SYBR GreenⅠ(Fig.1C).
The analytical sensitivity of T. vaginalis nested PCR and LAMP
The initial concentration of 90 ng/μL of T. vaginalis DNA was diluted by 101 -1012 times. As shown in Fig.2, the lowest template concentration was 90 × 10-7 ng/μL detected by nested PCR (Fig.2A and 2B), while that was 90 × 10-10 detected by LAMP amplification (Fig.2C and 2D). It could be seen that the analytical sensitivity of LAMP assays of T. vaginalis established in this study was 1000 times higher than that of nested PCR.
In order to further explore the sensitivity of LAMP amplification, the trophozoites of T. vaginalis were diluted to 103, 102, 101 and 1 respectively, and the DNA of these diluted samples was extracted. These results were shown that 103 trophozoites of T. vaginalis could be detected by nested PCR (Fig.3A and 3B), while 10 trophozoites of T. vaginalis could be detected by LAMP amplification (Fig.3C and 3D).
The analytical specificity of LAMP for T. vaginalis
There were no cross reactions in the LAMP using DNA extractions from T. vaginalis and other microorganisms including Trichinella spiralis, Toxoplasma gondii, Escherichia coli, Candida albicans, Staphylococcus aureus and Haemophilus. There were objective bands exclusively in experiments using DNA from T. vaginalis, either the results were observed under visible light by adding SYBR GreenⅠor using a UV transilluminator (Fig. 4).
As a kind of protozoan parasite that infects the genito-urinary system of human beings, T. vaginalis is found worldwide but receives less attention compared to other agents of STIs such as Neisseria gonorrhoeae and Chlamydia trachomatis [32-35]. From 2011 to 2014, the T. vaginalis prevalence in Granada, a capital city in Southern Spain was 2.4% [36]. According to the results of a cross-sectional research in a city attached to Yunnan Province, southern China, the T. vaginalis prevalence was 9.0% among 734 female sex workers [37]. In addition, according to an observation conducted in Xinxiang of Henan Province, China, 267 of 16294 (1.64%) samples from female patients suffering from certain trichomoniasis symptoms exhibited clinical positive results under wet mount microscopy [11].
Accurate and rapid diagnosis of trichomoniasis is the key process of treatment, prevention and blocking transmission. Generally, the methods used in detecting T. vaginalis in vaginal swabs are wet mount microscopy, culture, PCR, immunofluorescence and ELISA. However, there are disadvantages in these diagnostic methods [14]. In this study, the developed LAMP assay was a rapid and handy way to detect T. vaginalis with high analytical sensitivity and specificity, which was verified as superior to traditional nested PCR. Complicated equipment like thermal cycler was not necessary for LAMP, which could be conducted using hot water bath or common heating block. Moreover, the time for producing 109 target gene copies by the LAMP assay was no more than 3h, which could be reduced by half through the usage of additional loop primers,which was perfect for the point-of-care examinations demanding rapidness [27]. It was revealed by an orange-to-green color change due to adding SYBR GreenⅠthat large quantity of target gene copies were amplified successfully using LAMP [38]. The LAMP has been considered as a tool of cost-efficiency and rapidness for detecting numerous infections like HIV and malaria, although the potential value of which in detecting T. vaginalis hasn’t been developed up to now [39].
Previous researches have shown that LAMP has a 10 to 1000 fold lower limit of detection compared to conventional PCR [40-42]. A LAMP assay designed to detect Cyrptosporidium parvum was even proven to have a 100000 fold lower limit of detection compared to PCR [43]. The LAMP assay exhibited 1000 times higher sensitivity than the nested PCR in amplifying target genes of T. vaginalis. According to the results, the detecting limitation of LAMP was 10 trophozoites of T. vaginalis and that of nested PCR was as many as 103, and the difference was possibly due to the Bst DNA polymerase which was highly tolerate to inhibitors of nucleic acid amplification tests. Toye et al indicated that PCR was rarely inhibited using urine specimens, infrequently inhibited using endocervical swabs while frequently inhibited using urethral swabs [44]. Although the inhibiting effect could be reduced by various preparing approaches, it is not sufficient to eliminate the inhibitors of PCR from genital swabs by boiling the specimens. Moreover, for LAMP there was no decrease of signal intensity up to 100 trichomonads/mL and the bands in gel with stains of SYBR Safe exhibited typical ladder-like pattern, possibly resulting from significantly higher amplifying product quantity in comparison to that of PCR [38]. As complicated body fluid, urine and genital secretion had been applied to detecting T. vaginalis on the basis of nucleic acid, and the sensitivity of which were 64% - 100% for urine samples and 81% - 100% to genital secretion swabs [45, 46]. Previous studies have shown that LAMP reactions were not inhibited in spiked urine specimens [47]. Nevertheless, due to the usage of the wild type enzyme in the LAMP approach, unwanted activity of DNA polymerase in the process of setup possibly led to fail in reproducible amplification. In order to solve this problem, a warm start strand-displacing DNA polymerase which kept stable under ambient temperature while didn’t work until 50 °C was used by Tanner et al [48]. In our study, the time cost for performing LAMP of T. vaginalis with high analytical sensitivity from preparing samples to detecting LAMP products was no longer than 130 minutes.
Although some studies showed that LAMP could detect trichomonad based on target genes of actin, 18S rRNA and the 2-kbp repeated DNA, these genes have relatively high homology among different species [49-51]. AP65 is a prominent adhesin of T. vaginalis that mediates binding of parasites to host vaginal epithelial cells (VECs) [52]. We found that the sequences of AP65 had almost no homology with other species. Accordingly, AP65 as the target gene for detection possessed excellent specificity. In this current study, the LAMP of T. vaginalis was highly specific without crossreactivity to trichomonads of human beings with close relationship, such as Trichinella spiralis, Toxoplasma gondii, Escherichia coli, Candida albicans, Staphylococcus aureus and Haemophilus. Many previous studies shown that 6 primers were used for LAMP amplification of target genes [53, 54]. However, in the research, the 4 primers that recognized 6 instinct sites of the target gene led to the high specificity of LAMP, and AP65 gene could be detected specifically and sensitively without primers LF and LB. Therefore, the AP65 gene of T. vaginalis which was selected as the target gene for conducting highly specific LAMP could be used in the diagnosis of trichomoniasis [55, 56].
Nevertheless, there are a few shortages of LAMP. In spite of the high sensitivity and specificity, it is possible for the large quantity of DNA sequences obtained through the experiment to be contaminated by the opened tubes, which results in fault-positive consequences. In most cases, staining materials of nucleic acids , such as SYBR GreenⅠand Pico Green, are used in LAMP for detecting the product, while these materials exert an inhibiting effect on the amplifying process of LAMP. In addition, more than 1% contamination of biological substances such as blood and urine or more than 30% of saline solution or PBS can inhibit LAMP as well as PCR reactions [57]. Raw milk contaminants can even inhibit LAMP but not PCR. Consequently, using a real-time turbimeter to monitor the reaction in close tubes [38], using hydroxylnaphthol blue dye added in advance to conduct colorimetric determination [58], or adding wax barrier to SYBR GreenⅠ[59] are capable of preventing contamination due to opened tubes for visualizing endpoint results of LAMP.
The LAMP assay of T. vaginalis based on AP65 gene in the current work is convenient, specific, sensitive, and rapid way to detect trichomoniasis. However, this is a basic research, and more studies are needed in the future for verifying the diagnosing value of the LAMP assay of T. vaginalis in clinic. The valid and costeffective nucleic acid amplification test exhibits a promising potential in accurately diagnosing, extensively monitoring, effectively controlling and screening trichomoniasis in resource-limited and point-of-care settings.
TV: Trichomonas vaginalis (T. vaginalis); LAMP: Loop-mediated Isothermal Amplification; AP65: Adhesion Protein 65; PCR: Polymerase Chain Reaction; HIV: Human Immunodeficiency Virus; PBS: Phosphate Buffer Saline; ELISA: Enzyme Linked Immunosorbent Assay; TYM: Trypticase Yeast extract Maltose; NCBI: National Center for Biotechnology Information.
Ethics approval and consent to participate
The study was reviewed and approved by the Ethics Review Committee of the Xinxiang Medical University (Reference No. 2015016). The participants agreed that the vaginal secretions were used for this study and signed a consent form.
Consent for publication
Not applicable.
Competing interests
The authors declare that they have no competing interests.
Funding
This study was funded by the National Natural Science Foundation of China (No. 81802028) and the Doctoral Scientific Research Activation Foundation of Xinxiang Medical University (No. XYBSKYZZ201631 and XYBSKYZZ201504). The funders had no role in study design, data collection and analysis, decision to publish, or preparation of the manuscript.
Authors’ contributions
YHL and ZCZ conceived and designed the experiments. HZ and YD isolated and cultured the strain of T. vaginalis from the vaginal secretions. CYL and BLW extracted the DNA from T. vaginalis trophozoite. SFJ and QX performed nest-PCR. ZCZ designed the primers of LAMP. HRL and XXS performed LAMP. YHL and SW analyzed the data. ZCZ and YHL prepared the figures and tables. YHL wrote the paper. All authors read and approved the final manuscript.
Authors' information
1 Xinxiang Key Laboratory of Pathogenic Biology, School of Basic Medical Sciences, Xinxiang Medical University, Xinxiang, Henan, 453003, PR China.
Acknowledgements
Not applicable.
Availability of data and materials
All of the data in the present research are contained in the article.
Table 1 Oligonucleotide primer sequences used for Nested PCR in this research.
Name |
Sequences(5'-3') |
Description |
OUT-F |
TCTGGAATGGCTGAAGAAGACG |
Forward primer for the actin gene of T. vaginalis in the first stage |
OUT-R |
CAGGGTACATCGTATTGGTC |
Reverse primer for the actin gene of T. vaginalis in the first stage |
IN-F |
CAGACACTCGTTATCG |
Forward primer for the actin gene of T. vaginalis in the second stage |
IN-R |
CGGTGAACGATGGATG |
Reverse primer for the actin gene of T. vaginalis in the second stage |
AP65-FIP |
GCCGACATAGAAGGATGGGA CGCCCACTCAACCCAAAGGC |
Forward inner primer for the AP65 gene of T. vaginalis in LAMP assay |
AP65-BIP |
CCTCTACTCCTCTGGCCGTACAA ACTGTGTGGGAAACACCAT |
Backward inner primer for the AP65 gene of T. vaginalis in LAMP assay |
AP65-F3 |
CAACAGAGCACCCAGTTCTT |
Forward outer primer for the AP65 gene of T. vaginalis in LAMP assay |
AP65-B3 |
TGTGGAAGGGAGTAGCCTT |
Backward outer primer for the AP65 gene of T. vaginalis in LAMP assay |