key: cord-0075921-r3tpgz4r authors: Sukumolanan, Pratch; Demeekul, Kanokwan; Petchdee, Soontaree title: Development of a Loop-Mediated Isothermal Amplification Assay Coupled With a Lateral Flow Dipstick Test for Detection of Myosin Binding Protein C3 A31P Mutation in Maine Coon Cats date: 2022-03-07 journal: Front Vet Sci DOI: 10.3389/fvets.2022.819694 sha: 1c4d07f164b552ad2469fa3043dcb74877ad5f06 doc_id: 75921 cord_uid: r3tpgz4r BACKGROUND: Myosin-binding protein C3 A31P (MYBPC3-A31P) missense mutation is a genetic deviation associated with the development of hypertrophic cardiomyopathy (HCM) in Maine Coon cats. The standard detection of the MYBPC3-A31P mutation is complicated, time-consuming, and expensive. Currently, there has been a focus on the speed and reliability of diagnostic tools. Therefore, this study aimed to develop a loop-mediated isothermal amplification assay (LAMP) coupled with a lateral flow dipstick (LFD) test to detect MYBPC3-A31P mutations in Maine Coon cats. MATERIALS AND METHODS: Fifty-five Maine Coon cats were enrolled in this study, and blood samples were collected. MYBPC3-A31P was genotyped by DNA sequencing. Primers for LAMP with a LFD test were designed. The optimal conditions were determined, including temperature and time to completion for the reaction. The sensitivity of A31P-LAMP detection was compared between agarose gel electrophoresis (the standard method) and the LFD test. The A31P-LAMP-LFD test was randomly performed on seven cats (four with the A31P mutation and three wild-type cats). RESULTS: The A31P-LAMP procedure was able to distinguish between cats with MYBPC3-A31P wild-type cats and MYBPC3-A31P mutant cats. The LAMP reactions were able to be completed in 60 min at a single temperature of 64◦C. Moreover, this study demonstrated that A31P-LAMP coupled with the LFD test allowed for A31P genotype detection at a lower DNA concentration than agarose gel electrophoresis. DISCUSSIONS: This new A31P-LAMP with a LFD test is a successful and reliable assay with a rapid method, cost-effectiveness, and low requirements for sophisticated equipment for the detection of MYBPC3-A31P mutations. Thus, this assay has excellent potential and can be recognized as a novel screening test for hypertrophic cardiomyopathy associated with MYBPC3-A31P mutations in felines. Hypertrophic cardiomyopathy (HCM) is the most common hereditary cardiovascular disease in cats (1) (2) (3) (4) . The HCM phenotype has a prevalence of approximately 15% in cats (5) . Moreover, the HCM phenotype in cats is related to an increase in age. Cats with clinical HCM commonly demonstrated left-sided congestive heart failure due to an impairment of diastolic function such as respiratory distress, cardiogenic pulmonary edema, pleural effusion, syncope, hypothermia, and atrial thromboembolism (ATE) (6) (7) (8) (9) . Specific breeds are highly associated with HCM development, especially the Maine Coon (10) and Ragdoll (11) . Previous research investigated the cause of HCM in cats. Myosin binding protein C3 A31P (MYBPC3-A31P), a single nucleotide polymorphism (SNP), was possibly associated with HCM development in cats, especially Maine Coon cats (12) . MYBPC3, the sarcomeric protein in the myocardium, plays a crucial role in heart muscle contraction. Hence, MYBPC3-A31P mutation disturbs normal heart function and leads to cardiac concentric hypertrophy (12, 13) . The diagnosis of the HCM phenotype routinely relies on echocardiographic measurements. While detection of the SNP missense mutation MYBPC3-A31P is required for genetic screening in Maine Coon cats with familial HCM. However, cats without MYBPC3-A31P mutation may develop HCM. For the detection of SNP mutations, DNA sequencing is widely recognized as the gold standard technique (14) . However, due to the inconvenience of DNA sequencing, requiring laborintensive skills, prohibitive cost, and a long time, numerous researchers have developed different methods for SNP detection, such as allele-specific loop-mediated isothermal amplification (AS-LAMP) (15) , microarray genotyping (16) , molecular beacon genotyping (17) , allele-specific polymerase chain reaction (AS-PCR) (18) , and high-resolution melting (HRM) (19) . Based on advanced genetic research, LAMP is one of the accepted powerful methods for SNP detection. Applying a constant single temperature, LAMP can be used for point-of-care (POC) diagnostic tests owing to the utilization of simple instruments such as thermocyclers, heated blocks, or water baths. The advantages of LAMP are rapid detection with high accuracy because of four to six specific primers used for LAMP and isothermal amplification as a one-step process (20, 21) . In contrast, one disadvantage of LAMP is the challenge of designing a specific primer set. The detection of LAMP products is also usually performed by agarose gel electrophoresis. However, this method uses complex procedures and requires specialized equipment. The other commonly used methods for LAMP product verification are the visualization of colorimetric and lateral flow dipstick (LFD) tests, which are simple and straightforward for carrying out POC tests in a small animal hospital or small laboratory unit (22) . Nonetheless, the application of LAMP combined with LFD for the detection of MYBPC3-A31P mutations has not yet been reported. Therefore, this study aimed to develop a specific and rapid diagnostic tool for detecting MYBPC3-A31P mutations in Maine Coon cats using a LAMP assay coupled with an LFD. Fifty-five Maine Coon cats were recruited into this study. The procedures of animal use were permitted by Kasetsart University Institutional Animal Care and Use Committee, Kasetsart University, Bangkok, Thailand (Approval number: ACKU 62-VET-059). The blood samples were collected from venous vessels for 2-3 ml per cat and stored in an ethylenediaminetetraacetic acid (EDTA) tube. The stored blood was aliquoted and kept at −20 • C until DNA extraction. As described previously, the process of DNA extraction was conducted via Blood Genomic DNA Extraction Mini Kit (Favorgen, Taiwan) regarding manufacturer's recommendations (23) . The protocol for genotyping of MYBPC3-A31P mutation was obtained from a previous study by Godiksen et al. (24) . The details of forwarding and reverse primers were represented in Table 1 . In brief, the steps of PCR included heat activation at 95 • C for 15 min, 35 cycles of 3 steps of (i) denaturation at 95 • C for 30 s, (ii) annealing at 58 • C for 30 s, and (iii) extension at 72 • C for 1 min and final extension at 72 • C for 10 min. The size of the PCR product was 242 bp. PCR purification was then conducted following manufacturer's protocol (Favorgen, Taiwan). The Sanger sequencing was applied to determine the nucleotide of the MYBPC3 gene. The mutation of MYBPC-A31P was evaluated by using the Bioedit program. After MYBPC3-A31P genotyping, the enrolled cats were divided into two groups: wild-type genotype and mutant genotype. Three cats from the wild-type group and four cats from the mutant group were randomly selected, owing to the concentration and purity of DNA extraction for the detection of the A31P-LAMP method coupled with LFD test. The A31P-LAMP primer set was designed by using Primer Explorer version 5 software (http://primerexplorer.jp/lampv5e/ index.html). Based on our experience, the high guanine and cytosine (G/C) nucleotide in the sequence of the MYBPC3 required a manual design of the primer set. The DNA sequence of MYBPC3 protein was obtained from the National Center for Biotechnology Information (NCBI) database. In this research study, we designed the specific primer set based on the efficiency of recognition of SNP at position A31P for specifically selective amplification. The four designed primers can be used to detect mutant allele, cytosine (C), at the A31P missense mutation point from the MYBPC3. Four specific primers of A31P-LAMP, including forwarding inner primer (A31P-FIP), backward inner primer (A31P-BIP), A31P-F3 primer, and A31P-B3 primer were designed under the consideration of correlative comparable in the number of base pairs, percentage of G-C components, and melting temperatures. The position of MYBPC3-A31P was located at the 5' end of the designed forward inner primer (A31P-FIP). The designed primers set in this study were shown in Table 1 . The illustration of the MYBPC3, location of A31P-LAMP primer, and steps of the A31P-LAMP process are represented in Figure 1 . Frontiers in Veterinary Science | www.frontiersin.org optimal temperature of the A31P-LAMP reaction was evaluated at the gradient temperature, ranging from 60.8 to 68.0 • C. Moreover, the mixtures of LAMP reaction were experimented with to incubate with different time points for 30, 45, 60, and 75 min. After the A31P-LAMP protocol was optimized, an LFD test was conducted for validating the test efficacy. Regarding this study, the designed A31P-LAMP products were labeled with biotintagged BIP. In our experiment, an LFD test was performed according to commercial manufacture protocol (Melinia Genline HybriDetect, GieBen, Germany). In short, the amplificated A31P-LAMP product was added with 1 µM of A31P-probe which was labeled with a 6-carboxyfluorescein (6-FAM) probe and allowed to hybridize in the same temperature of A31P-LAMP amplification for 5 min. The sequence of designed A31P-probe is represented in Table 1 . Then, the 10 µl of hybridized LAMP products were directly dropped on lateral flow test strips. After that, lateral flow test strips were dipped into 80 µl of assay buffer that has been rewarmed at room temperature. Subsequently, the assay solution was emigrated by chromatography method along the test strips. The results of the LFD were observed by the naked eye within 5-15 min (Figure 2) . A positive result for the MYBPC3-A31P mutation was represented by two bands, the control line and the test line, appearing on the strip of the LFD test in a purple-red color. One band, the control line, appeared for homozygous wild-type cats. If no band appeared for the control line, the results of the LFD test were considered invalid. The analytical sensitivity of the A31P-LAMP test was determined in this study. The DNA of enrolled cats with MYBPC3-A31P mutation was diluted in various concentrations, including 10, 1, 0.1, 0.01, 0.001, 0.0001, and 0.00001 ng/µl. A31P-LAMP reaction was performed according to the protocol as described above. Then, the A31P-LAMP product was detected via (LFD test in comparison with a standard 1.5% agarose gel electrophoresis technique (25) . Table 2 . Figure 3 represents the DNA sequencing examination of the MYBPC3-A31P mutation. Design of the A31P-LAMP Primer for Detecting the MYBPC3-A31P Mutation In this study, we successfully designed a specific A31P-LAMP primer for detecting the mutant allele cytosine (C) of the MYBPC3-A31P mutation. MYBPC3-A31P is located at the 5' end of the forward inner primer (FIP) to distinguish between the wild-type genotype and mutant genotype in Maine Coon cats. The A31P-LAMP reaction on the MYBPC3-A31P mutation in cats is demonstrated in Figure 4 . The mutated allele (C), including the heterozygous mutation (G/C) (Lane 3) and the homozygous mutation (C/C) (Lane 4), was amplified and evaluated via agarose gel electrophoresis as the standard method. However, homozygous wild-type (G/G) was not able to be observed by A31P-LAMP detection. Therefore, the designed A31P-LAMP primer set is an excellent LAMP primer set for identifying the MYBPC3-A31P mutation. After designing an effective A31P-LAMP primer set, we sequentially optimized the conditions of the temperature and time to perform the A31P-LAMP reaction. The optimal temperatures were tested from 60.8 to 68.0 • C. We observed that A31P-LAMP was successful at 62.4 to 66.2 • C ( Figure 5A) . Thus, we selected the temperature of 64 • C as optimal for the A31P-LAMP reaction. Moreover, the time required for the A31P-LAMP reaction was optimized. We discovered that A31P-LAMP had positive results from 60 to 75 min ( Figure 5B) . Therefore, the A31P-LAMP reaction at 60 min provided a better experimental outcome based on the higher intensity signal on gel electrophoresis. A31P-LAMP coupled with the LFD test was operated to detect the designed LAMP products. Biotin was tagged at the backward inner primer (A31P-BIP) and 6-carboxyfluorescein (6-FAM) was labeled in the A31P-probe. In this experiment, two purplered color bands for the test line and control line appeared for mutant cats with either a heterozygous or homozygous mutation. However, only one band appeared at the control line in homozygous wild-type cats (Figure 6 ). Overall observations suggested that the A31P-LAMP coupled with the LFD test was potentially suitable for detecting MYBPC3-A31P. The sensitivity test of the designed A31P-LAMP reaction for detecting A31P-LAMP product was investigated using 10-fold serial dilutions of DNA concentration in comparison between agarose gel electrophoresis (standard method) and LFD test. In agarose gel electrophoresis, we found that the lowest DNA concentration to detect LAMP-A31P was 0.0001 ng/µl. In this study, seven out of 55 cats were diagnosed using the A31P-LAMP assay coupled with the LFD test, all seven cats were used in various DNA concentrations (from 0.0001 to 0.00001 ng/µl) to detect A31P mutation. The results showed that 0.00001 ng/µl of DNA concentration is the minimal amount that was able to detect A31P mutation with the LFD test in all seven cats (Figure 7) . The accumulated finding indicated that the LFD test provided more sensitivity to identify A31P-LAMP product than agarose gel electrophoresis. The MYBPC3-A31P mutation is of great concern in Maine Coon cats due to the severity of the pathogenesis and the HCM disease progression (26) . According to our findings in the recruited study animals, the MYBPC3-A31P mutation rate was 14.55%, which is low. In concordance with our recent prior publication, the mutation rates of MYBPC3-A31P and A74T in Maine Coon cats accounted for 21.43% in Thailand (23) . The prevalence of MYBPC3-A31P mutations worldwide (not included in Thailand) is around 34% (27) . Moreover, a study in a large European region showed that the prevalence of Maine Coon cats with the MYBPC3-A31P mutation was 41.5% (28) . To date, the gold standard for the detection of MYBPC3-A31P mutations is DNA sequencing. However, this method has various limitations, such as complicated processes, timeconsuming, a prohibitive cost, and requiring special equipment. Over the past few decades, many researchers have attempted to develop better techniques for detecting SNP gene mutations. There is currently no perfect screening test that can be applied as a simple diagnostic tool for SNP gene mutations, especially MYBPC3-A31P mutations in cats. This is the first study applying a LAMP coupled with an LFD test for screening MYBPC3-A31P mutations. Our findings demonstrated that A31P-LAMP associated with the LFD test can distinguish between wild-type cats and mutant cats with the MYBPC3-A31P mutation (Figure 6) . Nevertheless, this technique has some limitations due to its inability to differentiate between homozygous and heterozygous mutation carriers. After successfully developing a specific design of A31P-LAMP, the A31P-LAMP amplification was optimized for temperature and time (Figure 5) . We found that the designed A31P-LAMP can be amplified in wide ranges of temperatures and with various equipment, such as thermocyclers, heated blocks, and water baths. This is consistent with a previous study, where the researchers developed a LAMP for detecting the Mycobacterium leprae pathogen that causes Hansen's disease. The researchers were able to conduct LAMP amplification in both a heated block and a water bath (29) . Moreover, in this study, the average time to perform the MYBPC3-A31P test with LAMP was ∼110 min, including the process of DNA extraction, DNA amplification, and SNP detection. These data indicated that the designed A31P-LAMP required less time than other methods for SNP detection, such as PCR with DNA sequencing. PCR with DNA sequencing takes a long time due to the numerous steps, including DNA extraction, PCR, purification of PCR products, and DNA sequencing methods (30) . The designed A31P-LAMP can be clinically utilized as a rapid assay for MYBPC3-A31P mutation detection. To reduce the SNP detection time, in future studies, DNA from various samples, such as blood, dry blood spots (DBSs), hair follicles, or buccal swaps, will be extracted with sodium hydroxide (NaOH). This method can save time for DNA extraction owing to its simple DNA extraction procedure (31) . The LFD test is a widely accepted technique for detecting LAMP products. Following numerous lines of previous evidence, a LAMP assay combined with an LFD test was initially used for detecting several diseases not only in animals but also in humans. For instance, LAMP with the LFD test has been reported for use in the detection of the hepatitis B virus in human fields (32) . In this publication, the LAMP products were detected by agarose gel electrophoresis, LFD tests, and gold nanoparticles (AuNPs). The three methods had the same accuracy for hepatitis B virus detection. In humans infected with Plasmodium falciparum, LAMP with an LFD for specific SNP detection (Pf SNP-LAMP-LFD) was applied to investigate malarial disease. It has been reported that malarial disease is associated with antifolate molecular resistance to manage antimalarial drug strategies (33) . LAMP combined with LFD has been applied to detect hepatopancreatic parvovirus in shrimp (34) . They documented that this method is more sensitive than one-step PCR with agarose gel electrophoresis due to the lower DNA concentration. In terms of the objective of this study, the combination of LAMP with the LFD test had superior sensitivity for the detection of the designed LAMP product compared with agarose gel electrophoresis at 0.00001 ng/µl (Figure 7) . Based on these promising results, the designed A31P-LAMP coupled with the LFD test is a reliable assay for MYBPC3-A31P mutation screening. Similar to the previous study (35) , our results showed that the LAMP assay only took 110 min, this method provides on-site detection of a pathogen without requiring complex equipment. The LAMP assay is a rapid, simple, and sensitive test. Therefore, the A31P-LAMP assay could be more suitable as a screening point-of-care test for detecting the MYBPC3-A31P mutation in Maine Coon cats than the conventional PCR methods. In our pilot study, only 7/55 cats (12.73%) were diagnosed using the A31P-LAMP assay coupled with the LFD test, which was a limitation. For future work, it will be useful to increase the number of cats tested; however, we still gained valuable results by using the A31P-LAMP-LFD test in this study. Another limitation was that we did not investigate the efficacy of diagnostic examinations, such as the sensitivity and specificity, for MYBPC3-A31P diagnosis with the A31P-LAMP assay coupled with the LFD test. This should be further investigated in a larger population of Maine Coon cats. Novel methods for genetic testing of the MYBPC3-A31P mutation play a crucial role in reducing the effects of familial HCM in Maine Coon cats (26, 36) . According to the American College of Veterinary Internal Medicine (ACVIM) consensus statement guidelines for the classification, diagnosis, and management of cardiomyopathies in cats, MYBPC3-A31P screening is suggested to decrease the abnormal gene pool and reduce HCM development in Maine Coon cats (26, 36) . In this study, the A31P-LAMP method coupled with the LFD test is a rapid diagnostic tool for detecting MYBPC3-A31P mutations. Loop-mediated isothermal amplification for the MYBPC3-A31P mutation (A31P-LAMP) coupled with an LFD test has enormous potential for screening the crucial SNP mutation of the sarcomeric protein in Maine Coon cats with HCM. 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Prof. Dr. Janjira Phavaphutanon from the Department of Companion Animals Clinical Sciences, Kasetsart University for her advice and suggestions. Also, thanks to Kasetsart University Veterinary Teaching Hospital, Faculty of Veterinary Medicine, Kasetsart University and Biotechnology Laboratory, Kamphaeng Saen Veterinary Diagnostic Center, Faculty of Veterinary Medicine, Kasetsart University for providing the facilities for this research. The research was conducted with a patent application (ID: 2103003416).The authors declare that the research was conducted in the absence of any commercial or financial relationships that could be construed as a potential conflict of interest.