KR20180054160A - Primer set for multiple detection 4 kinds of virus infecting Passiflora edulis and method for detecting said viruses using the same - Google Patents

Abstract

The present invention relates to a primer set for multi-diagnosis of passion fruit infection viruses, and a diagnosis method using the same. The primer set comprises a primer pair represented by SEQ ID NO: 1 and SEQ ID NO: 2, a primer pair represented by SEQ ID NO: 3 and SEQ ID NO: 4, a primer pair represented by SEQ ID NO: 5 and SEQ ID NO: 6, and a primer pair represented by SEQ ID NO: 7 and SEQ ID NO: 8, and can perform multi-diagnosis of a Papaya leaf curl virus (PaLCuV), a Cucumber mosaic virus (CMV), a Euphobia leaf curl virus (EuLCV), and an East Asian Passiflora virus (EAPV). The primer set of the present invention can simultaneously diagnose four groups of viruses at once, and a time and costs consumed to diagnose viruses can be saved. Thus, economical feasibility is secured, and the present invention can contribute to production of virus disease-free stocks.

Description

TECHNICAL FIELD The present invention relates to a primer set for multiple diagnosis of four kinds of fungus infectious fungus viruses and a diagnostic method using the same.

The present invention relates to a primer set capable of simultaneously diagnosing four viruses infecting fashion fruity and a diagnostic method using the same.

About 20 viruses are known to infect fashion fruites worldwide, for example, Cowpea aphid-born mosaic virus , CABMV) or Passionfruit woody virus (PWV) cause woody to fruit. In particular, Papaya leaf curl virus (Papaya leaf curl virus, PaLCuV) , Cucumber Mosaic Virus (Cucumber mosaic virus, CMV), Lighthouse grass curl virus (Euphobia leaf curl virus, EuLCV) , and East Asia watch second virus (East Asian Passiflora virus, EAPV) is a virus that infects fashion fruity causing serious economic damage both at home and abroad. They are infected alone or in combination with fashionable fruids, and they cause great damage. Symptoms of these are mainly mosaic and leaf curl symptoms on the leaves, and other symptoms such as leaf spot, fruity lignification or deformity. In addition, when the viruses are infected, the quality of the fruit is deteriorated and the production amount is greatly influenced.

PaLCuV belongs to the genus Geminiviridae and Begomovirus , and has circular single stranded DNA. PaLCuV has a spherical particle shape, 18 nm in diameter, and a genome length of about 2.8 kb. PaLCuV was first reported in India in 1998 and has been reported to be able to infect papaya as a natural host and as an experimental host tobacco, petunia or tomato. PaLCuV causes leaf curl and stain symptoms on the leaves of fashion fruity. The PaLCuV is known to be a tobacco ( Bemisia tabaci ) and also spread to grafts.

CMV is a virus belonging to the genus Bromoviridae and Cucumovirus , and consists of three single stranded plus-sense RNAs. RNAs 1 and 2 of CMV produce the 1a and 2a proteins and are involved in the formation of replicase complexes. RNA 3 makes the 3a protein known as the viral movement protein (MP). CMV is infected by about 80 aphids. CMV, first discovered in cucumber in 1916, is now known to occur worldwide in all climates, including temperate and tropical, and can cause significant economic losses to about 1200 species of crops. CMV causes symptoms such as yellowing spots and mosaic of leaf, lignification and malformation of fruit in fashion fruity, and causes defective growth.

EuLCV belongs to the genus Geminiviridae and Begomovirus , and has circular single stranded DNA. The particle shape of EuLCV is double spherical, diameter is 18nm, and genome is 2.8kb. EuLCV is a natural host for tobacco ( Nicotiana tabacum ), tomato or poisonous euphorbia and poplaria ( Euphorbia pulcherrima ), and for the first time in 2014, infection has been reported in fashion fruiting.

EAPV is a virus belonging to the genus Potyviridae and Potyvirus, single-stranded positive-sense is composed of RNA. The length of the EAPV is 675-905 nm, and the genome is about 10 kb. EAPV is a non-persistent infection by aphids and was first discovered in fashion fruites. EAPV causes symptoms such as leaf blotches, mosaic, malformations or ligninization in the fashion fruity, causing bad growth and causing great damage to fashion fruit cultivation.

Viruses are pathogens smaller than 1 ㎛ in size and can not be observed with an optical microscope. They require an electron microscope to see them with the naked eye. And yet, there has not yet been developed a drug control method that directly affects viruses. In the past, electron microscopy and serological methods have been used for virus diagnosis. Electron microscopy can detect the presence of the virus, but it is impossible to diagnose it as a morphological feature. Among the serological methods, the enzyme-linked immunosorbent assay has a detection sensitivity about 1000 times lower than that of the most commonly used diagnostic methods or PCR methods, and fails to be diagnosed due to the unexpected nonspecific reaction of the antibody and the test sample Often occurs.

For this reason, precise and rapid diagnosis is a prerequisite for the management of viral diseases. On the other hand, reverse transcription-polymerase chain reaction (RT-PCR) method, which is commonly used for precise diagnosis in plant viruses, determines the specificity and accuracy of the diagnostic primer. In general, primers are designed to clone viruses and are not species specific. And sometimes produce nonspecific products of plants or other viruses, and thus are often unsuitable for diagnostic use. In addition, in order to diagnose various kinds of viruses in the same sample, there is a problem that many diagnosis cost and labor force are required by using various types of primers and performing reverse transcription-polymerase chain reaction respectively.

Korea is largely dependent on imports of fashion fruit seedlings, but the technology to accurately diagnose viruses that infect fashion fruids has yet to be found. Therefore, it is necessary to develop a technique for quickly and accurately diagnosing viruses that infect fashion fruites.

The present invention, both at home and abroad causing economically significant damage to the passion fruit papaya leaf curl virus (Papaya leaf curl virus, PaLCuV) , Cucumber Mosaic Virus (Cucumber mosaic virus, CMV) in order to solve the technical challenges, such as the lighthouse A pair of primers capable of specifically detecting Euphobia leaf curl virus (EuLCV) and East Asian Passiflora virus (EAPV) was designed, and RT- PCR) to select and provide a primer set that is highly sensitive to the virus.

The present invention also provides a virus diagnostic method and a diagnostic kit capable of detecting the viruses individually or simultaneously using a primer composition comprising the primer set.

In order to accomplish the above object, the present invention provides a primer pair comprising a pair of primers represented by SEQ ID NO: 1 and SEQ ID NO: 2, a pair of primers represented by SEQ ID NO: 3 and SEQ ID NO: 4, a pair of primers represented by SEQ ID NO: , and SEQ ID NO: 7 and papaya leaf curl virus (papaya leaf curl virus, PaLCuV), cucumber mosaic virus (cucumber mosaic virus, CMV) comprises at least two primer pairs selected from the group consisting of primer pair represented by SEQ ID NO: 8, There is provided a set of multiple RT PCR primers for diagnosing two or more fashion puffer viruses selected from the group consisting of Euphobia leaf curl virus (EuLCV) and East Asian Passiflora virus (EAPV).

The present invention also provides a primer pair represented by SEQ ID NO: 1 and SEQ ID NO: 2, a pair of primers represented by SEQ ID NO: 3 and SEQ ID NO: 4, a pair of primers represented by SEQ ID NO: 5 and SEQ ID NO: 6, papaya leaf curl, which includes a pair of primers represented by the number 8 virus (papaya leaf curl virus, PaLCuV) , cucumber mosaic virus (cucumber mosaic virus, CMV), lighthouse grass curl virus (Euphobia leaf curl virus, EuLCV) and East Asian clock seconds Provides a set of multiple reverse transcription PCR primers for the diagnosis of the virus of the East Asian Passiflora virus (EAPV).

The inventors of the present invention collected common nucleotide sequences in the above-mentioned four viruses and searched for common nucleotide sequences of all species and isolates of the species. Subsequently, by excluding the nucleotide sequences of other viruses that are related to each other in the common nucleotide sequence from the primer design, the species-specific sequences are selected, and the sequences having the optimal conditions as the primers from the species- As a primer. The combination of the above primers was subjected to an actual RT-PCR (RT-PCR), and a combination with no sensitivity to nucleic acids other than the target virus and excellent sensitivity to the target virus was finally selected to complete the present invention .

The primers of the present invention were developed to allow RT-PCR products to be synthesized species-specifically for the virus. In the present invention, the term "species-specific" means that the primer can synthesize a specific RT-PCR product from the genomic sequence of the virus to be diagnosed, and it is common for all the strains in the virus species to be diagnosed And nonspecific reactions with nucleic acids derived from other similar species or plants should not occur. Generally used primers are designed to amplify specific genes of viruses and are not species specific, and are sometimes unsuitable for diagnostic use because they may produce nonspecific products by the nucleic acid of plants or other viruses .

Specifically, the primer of the present invention was designed in the following manner. (a) selecting the target genome of the target virus; (b) search for common sequences in known strains of viruses and isolate genomic sequences to date; (C) excluding the same or similar sequence as the genome of a similar virus; (d) A primer was designed by selecting only a base sequence capable of functioning as a primer. A pair of primers that can be subjected to species-specific amplification by RT-PCR among the designed primers and which does not cause nonspecific reaction was selected.

In the present invention, a 'primer' is a nucleic acid sequence having a short free 3 'hydroxyl group and can form base pairs with a template of a complementary nucleic acid. Quot; means a short nucleic acid sequence which functions as a starting point. The primers can initiate DNA synthesis in the presence of reagents and four different nucleoside triphosphates for polymerization reactions (i. E., DNA polymerase or reverse transcriptase) at appropriate buffer solutions and temperatures.

In order to distinguish the four viruses from each other by RT-PCR electrophoresis, it was necessary to distinguish the sizes of the viruses. Therefore, considering the size of amplified product, a pair of primers for detecting each virus was selected.

For the PaLCuV detection, primer pairs shown in SEQ ID NOS: 1 and 2, primer pairs shown in SEQ ID NOS: 3 and 4 for CMV detection, primer pairs shown in SEQ ID NOS: 5 and 6 for EuLCV detection, For the detection, primer pairs shown in SEQ ID NOS: 7 and 8 were used.

A sample infected with the selected primer pairs PaLCuV, CMV, EuLCV and EAPV alone, two kinds of compound infections, three kinds of compound infections, four kinds of compound infections, and four kinds of complex infections was subjected to RT-PCR and the products were subjected to electrophoresis, The viruses were distinguishable by size. Therefore, it can be seen that the above primer pair can be useful for diagnosing the four viruses simultaneously or individually.

According to another embodiment of the present invention, the present invention provides one or more fashion puffer virus diagnostic kits selected from the group consisting of PaLCuV, CMV, EuLCV and EAPV including the primer set.

In addition, the present invention provides a composition for multiple diagnosis of PaLCuV, CMV, EuLCV and EAPV comprising the primer set and a kit comprising the same.

The composition means a reagent, a thermostable DNA polymerase, a dNTP and a solution containing a divalent metal cation necessary for performing an RT-PCR amplification reaction.

The kit includes a primer pair shown in SEQ ID NO: 1 and 2, a primer pair shown in SEQ ID NO: 3 and 4, a primer pair shown in SEQ ID NO: 5 and 6, and SEQ ID NO: 7 and 8 One or more primer pairs selected from the group consisting of a pair of primers and a reagent for performing a reverse reaction and an amplification reaction. The reagent for carrying out the amplification reaction in the kit may include reverse transcriptase, DNA polymerase, dNTPs, buffer, and the like. In addition, components necessary for conducting electrophoresis to confirm whether the RT-PCR product is amplified can be further included in the kit of the present invention. Further, it may contain an RNase inhibitor, DEPC-water, sterilized water and the like if necessary.

In the present invention, 'RT-PCR kit' can be prepared by putting the RT-PCR composition into a plastic tube in a lyophilized form, and the kit further includes appropriate reagents and tools used for analysis in addition to the RT-PCR composition Such reagents and tools may include suitable carriers, labels capable of generating detectable signals, solubilizers, detergents, and the like.

Such suitable carriers include, but are not limited to, soluble carriers such as physiologically acceptable buffers known in the art such as PBS, insoluble carriers such as polystyrene, polyethylene, polypropylene, polyester , Polyacrylonitrile, fluorine resin, crosslinked dextran, polysaccharide, polymer such as magnetic fine particles plated with metal on latex, other paper, glass, metal, agarose, and combinations thereof.

(A) separating the viral RNA from the sample; (b) a primer pair shown in SEQ ID NO: 1 and SEQ ID NO: 2, a primer pair shown in SEQ ID NO: 3 and SEQ ID NO: 4, SEQ ID NO: 5 and SEQ ID NO: 6 And a primer pair shown in SEQ ID NO: 7 and SEQ ID NO: 8; And (c) separating the RT-PCR products of step (b) by size. The method of claim 1, wherein the RT-PCR product is selected from the group consisting of PaLCuV, CMV, EuLCV and EAPV.

Preferably, the present invention provides a method of detecting a virus, comprising: (a) separating viral RNA from a sample; (b) a primer pair shown in SEQ ID NO: 1 and SEQ ID NO: 2, a primer pair shown in SEQ ID NO: 3 and SEQ ID NO: 4, SEQ ID NO: 5 and SEQ ID NO: 6 And a primer pair shown in SEQ ID NO: 7 and SEQ ID NO: 8; And (c) separating the RT-PCR products of step (b) by size.

The RNA extraction in the step (a) may be performed according to a method commonly used in the art, and may be carried out using a commercially available RNA extraction kit.

In addition, in the step (b), the cDNA strands were synthesized by reverse transcription using reverse transcriptase, using the RNA isolated as the template in step (a) as a template and the reverse primer of the primer pair of the present invention as a primer Next, the PCR reaction mixture may be used. The PCR reaction may be performed using a PCR reaction mixture containing various components known in the art necessary for the PCR reaction. In the PCR reaction mixture, a suitable amount of DNA polymerase, dNTP, PCR buffer solution and water are contained in addition to the cDNA synthesized by the reverse transcription reaction and the primer pair provided in the present invention. The PCR buffer solution may include Tris-HCl, MgCl ₂ , KCl, and the like. At this time, the MgCl ₂ concentration greatly affects the specificity and yield of amplification. Generally, when Mg ^{2 +} is excessive, nonspecific PCR amplification product is increased, and when Mg ^{2 +} is insufficient, the yield of PCR product is decreased . The PCR buffer solution may further contain an appropriate amount of Triton X-100 (Triton X-100). Also, PCR was performed by denaturing the template DNA at 94-95 ° C, followed by denaturation; Annealing; Followed by a cycle of amplification and extension followed by final elongation at 72 ° C. Modification and amplification may be performed at 94-95 ° C and 72 ° C, respectively, and the temperature at the time of binding may vary depending on the type of the primer, but is preferably 50-57 ° C, more preferably 55 ° C . The time and number of cycles in each step can be determined according to the conditions commonly practiced in the art.

In the step (c), the DNA of the PCR product can be isolated by size according to a method well known in the art. Preferably by agarose gel or polyacrylamide gel electrophoresis or an ABI prism 3100 genetic analyzer-electropherogram. In this case, in order to use the fluorescence analyzer, PCR is performed in step (b) using a pair of primers having a fluorescent dye well known in the art.

The PCR amplification result can preferably be confirmed by agarose gel electrophoresis. After electrophoresis, electrophoresis results can be analyzed by ethidium bromide staining. Methods for performing general reverse transcription, PCR and analysis of the results are well known in the art.

The primer set for the diagnosis of fashion puffer virus according to the present invention can not only diagnose PaLCuV, CMV, EuLCV and EAPV but also simultaneously diagnose two or more viruses at the same time.

Through the primer set, it is possible to diagnose the infection of the fashion fruit virus early, thereby preventing the economic loss of the farmhouse due to the infection.

The use of the primer set according to the present invention makes it possible to accurately and specifically diagnose the fashionable virus.

The multi-diagnosis method of the present invention can reduce the cost and time required for diagnosis of fashion fruit viruses and is economical and can be effectively used for the development of disease free production of fashion fruit viruses.

FIG. 1 is a photograph showing a main symptom of a fungus infectious virus.
Figure 2 shows the RT-PCR test results of PaLCuV diagnostic primer combinations.
Figure 3 shows RT-PCR results of the primer combination for CMV diagnosis.
Figure 4 shows the results of RT-PCR assays for the EuLCV diagnostic primer combination.
Figure 5 shows RT-PCR results of primer combinations for EAPV diagnosis.
FIG. 6 shows the result of RT-PCR of the combination of PaCluV, CMV, EuLCV and EAPV alone or two or more diagnostic primers (M: 100 bp ladder, 1: EAPV, 2: EuLCV, 3: CMV, 4: PaLCuV EAPV + EuLCV, 6: EAPV + CMV, 7: EAPV + PaLCuV, 8: EuLCV + CMV, 9: EuLCV + PaLCuV, 10: CMV + PaLCuV, 11: EAPV + EuLCV + CMV, 12: EAPV + EuLCV EAVV + EuLCV + CMV + PaLCuV, M: 100 bp ladder)

Hereinafter, embodiments of the present invention will be described in detail to facilitate understanding of the present invention. However, the embodiments according to the present invention can be modified into various other forms, and the scope of the present invention should not be construed as being limited to the following embodiments. Embodiments of the invention are provided to more fully describe the present invention to those skilled in the art.

Example 1: Establishment of a fashion puffer virus detection system

The diagnostic primers of PaLCuV, CMV, EuLCV and EAPV, which infect fashion fruids at home and abroad, were designed with reference to previously reported nucleotide sequences. Only the primers that specifically reacted with the target virus were selected.

1-1. PaLCuV diagnostic primer selection

PaLCuV diagnostic primers were designed for two pairs of sizes 569 bp and 605 bp for the V1, V2 and C3 regions, which are shown in Table 1. As a result of the RT-PCR test on PaLCuV conjugated samples, both pairs were selected as specific primers for PaLCuV diagnosis. The primers used in the following Table 2 are shown and RT-PCR results are shown in FIG.

Name of the primer Locus The sequence (5 '- > 3') Expected size PaLCuV-m-1F 539-558 AAGGTCCTTTGTGTCTCCGA 569 bp PaLCuV-m-1R 1108-1091 CGATGTATTAGTCGGAAC PaLCuV-m-2F 254-271 CTGTCTTACGTGCAAGGA 605 bp PaLCuV-m-2R 856-837 GCTTGCATATTGACCACCAG

Lane Sample No. Primer used One One PaLCuV-m-1F PaLCuV-m-1R 2 PaLCuV-m-2F PaLCuV-m-2R

1-2. CMV diagnostic primer selection

The CMV diagnostic primer was designed for a coat protein (CP) pair of 473 bp in size, as shown in Table 3. As a result of an RT-PCR test on a single infected sample of CMV, the above pair was selected as a specific primer for CMV diagnosis, and the results are shown in Table 4 and FIG.

Name of the primer location The sequence (5 '- > 3') Expected size CMV DP u1 1307-1325 CGTCGTGGTTCCCGCTCCG 473bp CMV DP d2 1780-1761 AGCGCGCATCGCCGAAAGAT

Lane Sample No. Primer used One One CMV 1-2 u CMV 1-2 d 2 2 3 3 4 N 5 P

1-3. Selection of EuLCV diagnostic primer

The EuLCV diagnostic primer was designed for a pair of size 342 bp in the V2 region, which is shown in Table 5. As a result of an RT-PCR test on EuLCV-infected samples, the pair was selected as a specific primer for EuLCV diagnosis, and the results are shown in Table 6 and FIG.

Name of the primer Locus The sequence (5 '- > 3') Expected size EuLCV-F 26-46 AGTGGTCCCCCCTCCA (C) CTAAC 342 bp EuLCV-R 367-348 CAGCCTCCGTCGAACCTTCG

Lane Sample No. Primer used One One EuLCV-F EuLCV-R 2 2

1-4. EAPV diagnostic primer selection

EAPV diagnostic primers were designed for two pairs of size 231 bp and 220 bp, respectively, in the coat protein (CP) region and are shown in Table 7. As a result of the RT-PCR test for the single infected sample of EAPV, the above two pairs were selected as specific primers for EAPV diagnosis, and the results are shown in Table 8 and FIG.

Name of the primer Locus The sequence (5 '- > 3') Expected size EAPV-IB-1F 9423-9433 CATTGATAATGGCACCTCACC 231 bp EAPV-IB-1R 9654-9635 AGCCAAACTCAAGTCCCTCA EAPV-IB-2F 9320-9339 CGACCAAATCACAGTTCGAG 220bp EAPV-IB-2R 9540-9521 CTGTCTCAGAGTGGGCTGAG

Lane Sample No. Primer used One One EAPV-IB-1F EAPV-IB-1R 2 One EAPV-IB-2F EAPV-IB-2R

Example 2: Development of multiple diagnosis methods for four kinds of viruses occurring in fashion fruites

Among the specific diagnostic primers designed for the fashion fruit viruses PaLCuV, CMV, EuLCV and EAPV, multiple diagnostic primers as shown in Table 9 below were selected for simultaneous diagnosis of four viruses by one RT-PCR. We have developed a multiplex RT-PCR method that can diagnose the fashion puffer virus PaLCuV, CMV, EuLCV and EAPV at once.

virus Name of the primer The sequence (5 '- > 3') location Expected size density PaLCuV PaLCuV-m-2F CTGTCTTACGTGCAAGGA (SEQ ID NO: 1) 289-306 605bp 50 pmol PaLCuV-m-2R GCTTGCATATTGACCACCAG (SEQ ID NO: 2) 893-873 CMV CMV 1-5 u CTTGTGCGTTTRATGGCTACGAAGGC (SEQ ID NO: 3) 2646-3283 473bp 30 pmol CMV 1-5 d CACGGACCGAAGTCCTTCCGAAGAAA (SEQ ID NO: 4) 3284-3259 EuLCV EuLCV-F AGTGGTCCCCCCTCCA (C) CTAAC (SEQ ID NO: 5) 26-46 342bp 40 pmol EuLCV-R CAGCCTCCGTCGAACCTTCG (SEQ ID NO: 6) 367-348 EAPV EAPV-IB-1F CATTGATAATGGCACCTCACC (SEQ ID NO: 7) 9423-9433 231 bp 40 pmol EAPV-IB-1R AGCCAAACTCAAGTCCCTCA (SEQ ID NO: 8) 9654-9635

For the diagnosis of PaLCuV, CMV, EuLCV and EAPV, primers selected from the above were used. In the case of the fashion puffer samples, the leaves with the symptoms were ground with liquid nitrogen, and then the entire genome was extracted using a total RNA extraction kit (Intron Co.).

1 μl of genomic template, 0.5 μl of forward primer (30-50 pmol), 0.5 μl of reverse primer (30-50 pmol), 8 μl of distilled water and 10 μl of RT-PCR premix were added to the final 20 μl As a reaction solution.

DNA was subjected to initial denaturation at 94 ° C for 3 min, followed by 35 cycles of 94 ° C for 20 sec for denaturation of DNA, 30 sec for 55 ° C for primer annealing and 1 min at 72 ° C for DNA chain extension, . The products were amplified by PCR with PaLCuV, CMV, EuLCV and EAPV at 72 ° C for 10 min for DNA chain extension. The product was confirmed by electrophoresis on 1.2% agarose gel, 100mV for 1 hour 30 minutes.

As shown in FIG. 6, the results of both the single infection and the combined infection showed a correct response, and the magnitude of the amplification sequence was also markedly different. Accordingly, it has been found that four types of viruses occurring in fashion fruites can be diagnosed accurately simultaneously by using the primer set of the present invention.

<110> REPUBLIC OF KOREA (MANAGEMENT: RURAL DEVELOPMENT ADMINISTRATION) <120> Primer set for multiple detection 4 kinds of virus infecting          Passiflora edulis and method for detecting said viruses using the          same <130> P16-282 / 2016-0493-10-A <160> 8 <170> KoPatentin 3.0 <210> 1 <211> 18 <212> DNA <213> Artificial Sequence <220> <223> PaLCuV-m-2F <400> 1 ctgtcttacg tgcaagga 18 <210> 2 <211> 20 <212> DNA <213> Artificial Sequence <220> <223> PaLCuV-m-2R <400> 2 gcttgcatat tgaccaccag 20 <210> 3 <211> 26 <212> DNA <213> Artificial Sequence <220> <223> CMV 1-5 u <400> 3 cttgtgcgtt tratggctac gaaggc 26 <210> 4 <211> 26 <212> DNA <213> Artificial Sequence <220> <223> CMV 1-5 d <400> 4 cacggaccga agtccttccg aagaaa 26 <210> 5 <211> 22 <212> DNA <213> Artificial Sequence <220> <223> EuLCV-F <400> 5 agtggtcccc cctccaccta ac 22 <210> 6 <211> 20 <212> DNA <213> Artificial Sequence <220> <223> EuLCV-R <400> 6 cagcctccgt cgaaccttcg 20 <210> 7 <211> 21 <212> DNA <213> Artificial Sequence <220> <223> EAPV-IB-1F <400> 7 cattgataat ggcacctcac c 21 <210> 8 <211> 20 <212> DNA <213> Artificial Sequence <220> <223> EAPV-IB-1R <400> 8 agccaaactc aagtccctca 20

Claims (6)

A pair of primers represented by SEQ ID NO: 1 and SEQ ID NO: 2, a pair of primers represented by SEQ ID NO: 3 and SEQ ID NO: 4, a pair of primers represented by SEQ ID NO: 5 and SEQ ID NO: 6, and a pair of SEQ ID NO: that papaya leaf curl virus comprises at least two primer pairs selected from the group consisting of a pair of primers (papaya leaf curl virus, PaLCuV) , cucumber mosaic virus (cucumber mosaic virus, CMV), lighthouse grass curl virus (Euphobia leaf curl virus, EuLCV ) And East Asian Passiflora virus (EAPV). &Lt; / RTI &gt; A pair of primers represented by SEQ ID NO: 1 and SEQ ID NO: 2, a pair of primers represented by SEQ ID NO: 3 and SEQ ID NO: 4, a pair of primers represented by SEQ ID NO: 5 and SEQ ID NO: 6, and a pair of SEQ ID NO: that papaya leaf curl virus containing a pair of primers (papaya leaf curl virus, PaLCuV) , cucumber mosaic virus (cucumber mosaic virus, CMV), lighthouse grass curl virus (Euphobia leaf curl virus, EuLCV) and East Asia watch second virus (East Asian Passiflora virus , EAPV) for the diagnosis of fashionable viruses. A kit for diagnosing one or more fashion puffer viruses selected from the group consisting of PaLCuV, CMV, EuLCV and EAPV comprising the primer set of claim 1 or 2. Papaya leaf curl including the primers represented by the nucleotide sequence of SEQ ID NO: 1 to 8 virus (Papaya leaf curl virus, PaLCuV) , cucumber mosaic virus (Cucumber mosaic virus, CMV), lighthouse grass curl virus (Euphobia leaf curl virus, EuLCV ) And East Asian Passiflora virus (EAPV). A kit comprising the composition of claim 4. (a) separating the viral RNA from the sample;
(b) using the RNA of step (a) as a template,
A pair of primers represented by SEQ ID NO: 1 and SEQ ID NO: 2, a pair of primers represented by SEQ ID NO: 3 and SEQ ID NO: 4, a pair of primers represented by SEQ ID NO: 5 and SEQ ID NO: 6, and a pair of SEQ ID NO: Performing RT-PCR using a primer pair that is a primer pair; And
(c) separating the RT-PCR product of step (b) by size, wherein the method comprises the steps of: (a) isolating the RT-PCR product of step (b)

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