CN108715899B - Aeromonas veronii detection primer, kit, detection method and development method thereof based on specific sequence - Google Patents

Aeromonas veronii detection primer, kit, detection method and development method thereof based on specific sequence Download PDF

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CN108715899B
CN108715899B CN201810349016.1A CN201810349016A CN108715899B CN 108715899 B CN108715899 B CN 108715899B CN 201810349016 A CN201810349016 A CN 201810349016A CN 108715899 B CN108715899 B CN 108715899B
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刘柱
马香
唐燕琼
唐鸿倩
胡新文
杜明伦
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Abstract

The invention relates to a primer pair for detecting Aeromonas veronii, wherein the nucleotide sequence of a forward primer of the primer pair is selected from SEQ ID NO.1 and/or SEQ ID NO.3, and the nucleotide sequence of a reverse primer of the primer pair is selected from SEQ ID NO.2 and/or SEQ ID NO. 4. The invention also relates to a reagent and a kit containing the primer pair or the primer pair combination and application of the reagent and the kit in detecting Aeromonas veronii. The invention also relates to a method for developing primers for detecting Aeromonas veronii.

Description

Aeromonas veronii detection primer, kit, detection method and development method thereof based on specific sequence
Technical Field
The invention relates to an Aeromonas veronii detection primer based on a specific sequence, a reagent containing the primer, a kit, an Aeromonas veronii detection method and a method for developing the Aeromonas veronii detection primer, and belongs to the field of molecular biology.
Background
Aeromonas veronii (Aeromonas veronii), also known as Aeromonas veronii, and Aeromonas veronii, is a gram-negative rod-shaped bacterium belonging to the spore-free facultative anaerobic type. The bacteria are distributed in distributed manner, are commonly present in fresh water, sewage, soil or even seawater, are blunt-rounded at both ends, have a size of about 0.3-0.7. mu. m.times.1.2-2.5. mu.m, have flagella, and are mobile (Kirov SM, Tassell BC, sembler AB, O' Donovan LA, Rabaan AA et al. "Lateral flagella and swarming mobility in Aeromonas species" [ J ]. J Bacteriol.2002,184(2): 547-555).
Aeromonas veronii belongs to a virulent pathogen, the pathogenic process mainly comprises adhesion-invasion-in-host colonization and toxin secretion processes, and a series of virulence factors such as aerolysin, enterotoxin and adhesion factor are generated during the pathogenic process, and the virulence factors play a role in the weight bearing of aquatic animals, human beings and even livestock and poultry infection (Yuan, Wang Kai, Chende Fang, Huang Ling and Wang equalling. "research on tissue localization and dynamic distribution of Aeromonas veronii in artificially infected channel catfish" [ C ]. the twenty-ninth academic conference corpus of fishery forum in south China, Guangxi North sea, 2013).
The host infection range of the bacterium is very wide. First, this bacterium is one of the oldest known fish pathogens, infects many kinds of freshwater fish, marine fish, etc., and poses a serious threat to aquaculture fish and wild fish (Bossi-Kpfer M, Genini A, Peduzzi R, demanta A. "Trachelenchitis used by Aeromonas veronii biovar sobriear after water-lowering" [ J ]. J Med Microbiol.2007,56(Pt 11): 1563-. For example, when a grass carp is infected with aeromonas veronii, local hemorrhage, ascites, splenomegaly and other symptoms (Wang Hao, quan Zi, Li Meng Ying, Lu Li Tu., "the medication of enrofloxacin to control aeromonas veronii of grass carp" [ J ]. freshwater fishery, 2013,43(2): 47-53).
Meanwhile, aeromonas veronii can also infect arthropods and reptiles, such as eriocheir sinensis (sea, cheng cuizhen, zhang jun yun, ge xian xiang. "test of aeromonas veronii as a pathogen of eriocheir sinensis" [ J ]. proceedings of zoonosis of china [ 2008,24(1):45-49), and trionyx sinensis (qiang ming. "research on isolation, identification and prevention of the pathogen of death disease of trionyx sinensis group" [ D ]. major thesis of north river university, 2010), etc. In addition, the bacterium can also cause infectious complications in mice and normal and immunocompromised persons, causing a variety of infectious conditions including arthritis, wound infection, gastroenteritis, bacteremia, meningitis and endocarditis (Lye DJ. "scientific infection rates for human clinical laboratories" [ J ]. Curr Microbiol.2011,63(4): 332-.
In recent years, increasing cases have shown that aeromonas veronii has become an important human-fish co-pathogenic bacterium, which is widely distributed, highly pathogenic, and has a prominent position in food safety, and some countries have specified it as a subject of food safety quarantine (wu shang base, daemon dawden, mengqing peak, guoweishen, wangweili, qiandong, etc.. "progress in aeromonas veronii research" [ J ]. magazine of chinese veterinary drugs, 2011(07): 41-44).
Currently, the identification and detection method of Aeromonas veronii relies mainly on conventional physiological and biochemical tests designed according to the nutritional requirements and metabolites of the bacteria, but this method is time consuming, laborious and unreliable in results (Lamyb, Laurent F, Verdier L et al. "acquisition of 6Commercial Systems for identifying Clinical Aeromonas Isolates" [ J ]. Diagnostic Microbiology and Infections Disease 2010,67: 9-14). The detection of Aeromonas veronii is also dependent on common bacteriological methods such as apparent pathological observation and bacteria separation and identification, but the pathological phenomena of diseases caused by Aeromonas veronii are very similar to other Aeromonas veronii and difficult to judge by naked eyes, and the conventional bacteria separation and identification is time-consuming and labor-consuming. In addition, molecular biological and immunological methods can also be applied. Molecular biological methods are based on the identification of bacteria and their classification based on the Length and sequence variation of Specific conserved sequences, such as 16S rDNA ("A DNA Probe specificity for Aeromonas colloids" [ J ]. Diagnostic Microbiology and Infectious Disease,2002,44: 221-.
In addition, the variety of ISRs of Aeromonas veronii is large, which is not beneficial to detection, and research has shown that the ISRs of Aeromonas veronii have high similarity (LAGANOSKA M, KAZNOWSKI A. "research fragment length polymorphism of 16S-23SrDNA interactive spacer of Aeromonas pp" [ J ] Syst Appl Microbiol,2004,27(5): 549-.
As can be seen, the molecular biological identification method of Aeromonas veronii is not yet mature. Immunological Methods, i.e.the detection of bacterially specific antigenic proteins by means of specific enzyme-linked immunosorbent assays (ELISA), have not been investigated sufficiently, and a large number of antigens capable of specifically identifying Aeromonas veronii (Arora S, Agarwal R K, Bist B. "comprehensive of ELISA and PCR vis-a-vis clinical Methods for Detecting Aeromonas spp. in Foods of animal Origin" [ J. International Journal of Food Microbiology,2006,106:177-183)
Thus, in general, the detection of Aeromonas veronii is still in a lag phase, so that when aquatic animals, especially humans, are infected with pathogenic bacteria, misdiagnosis often occurs, often with serious consequences-massive death of the cultured aquatic animals and persistent or even death of the patients.
Therefore, the development of a method capable of rapidly and simply detecting Aeromonas veronii is a key and important point for the prevention and treatment of diseases caused by Aeromonas veronii in the future.
Disclosure of Invention
The invention aims to provide a primer pair for detecting Aeromonas veronii, which has strong specificity and high sensitivity and can quickly and accurately detect the Aeromonas veronii.
Another object of the present invention is to provide a reagent or a kit for detecting Aeromonas veronii, which is highly sensitive, rapid, simple and inexpensive.
Another object of the present invention is to provide a method for detecting Aeromonas veronii, which can rapidly, conveniently and accurately identify the presence of Aeromonas veronii using the above primer pair, reagent or kit of the present invention.
Alternatively, another object of the present invention is to provide the use of the above primer pair, reagent or kit of the present invention in the preparation of a detection agent for detecting the presence of Aeromonas veronii, whereby the presence of Aeromonas veronii can be identified quickly, conveniently and accurately.
It is still another object of the present invention to provide a method for developing a primer for detecting Aeromonas veronii, thereby providing a primer that has strong specificity, high sensitivity, and can rapidly and accurately detect Aeromonas veronii.
The first aspect of the present invention provides a primer pair for detecting Aeromonas veronii, wherein:
(1) the nucleotide sequence of the forward primer of the primer pair is selected from one or more of the following: the nucleotide sequence shown in SEQ ID NO.1, the nucleotide sequence shown in SEQ ID NO.3 and the nucleotide sequence generated by substituting, deleting and/or adding one or more nucleotides in the nucleotide sequence shown in SEQ ID NO.1 or SEQ ID NO. 3; and
(2) the nucleotide sequence of the reverse primer of the primer pair is selected from one or more of the following: the nucleotide sequence shown in SEQ ID NO.2, the nucleotide sequence shown in SEQ ID NO.4 and the nucleotide sequence generated by substituting, deleting and/or adding one or more nucleotides in the nucleotide sequence shown in SEQ ID NO.2 or SEQ ID NO. 4.
In one embodiment, the primer pair of the present invention is selected from any one of the following (1) to (2):
(1) the nucleotide sequence of a forward primer of the primer pair WP _041202667.1 is shown as SEQ ID NO.1, and the nucleotide sequence of a reverse primer of the primer pair WP _041202667.1 is shown as SEQ ID NO. 2;
(2) the nucleotide sequence of a forward primer of the primer pair WP _041202667.1_ par is shown as SEQ ID NO.3, and the nucleotide sequence of a reverse primer of the primer pair WP _041202667.1_ par is shown as SEQ ID NO. 4;
or any combination thereof.
In one embodiment, one of the primers in the primer pair is detectably labeled. Labeling methods are well known in the art. The label includes those commonly used in the art, for example, the label includes, but is not limited to, a radioisotope, an enzyme, a fluorescent substance, a luminescent substance, biotin, or the like. Preferably, the label is a fluorescent label, more preferably, the fluorescent label includes, but is not limited to, FAM, HEX, TAMRA, ROX, and like fluorescent dyes. In further embodiments, the forward primer of the primer pair is labeled, or the reverse primer of the primer pair is labeled. In another embodiment, the primer may be modified by any modification means known to those skilled in the art to change, thereby improving the specificity of the primer and/or facilitating detection of the primer.
In a second aspect, the present invention provides a reagent for detecting Aeromonas veronii, the reagent comprising any of the primers of the present invention described above. In one embodiment, each pair of primers contained in the reagent of the present invention is packaged separately.
In a third aspect, the present invention provides a kit for detecting Aeromonas veronii, the kit comprising any of the primers or reagents described herein above.
In one embodiment, the kit of the invention further comprises at least one fluorescent probe, such as a TaqMan probe, a FRET hybridization probe (fluorescence resonance energy transfer probe) and a molecular beacon. In a preferred embodiment, the fluorescent probe is a TaqMan probe designed between the primers of the present invention based on SEQ ID NO.5 or SEQ ID NO. 7. Methods for designing TaqMan probes are known to those skilled in the art.
In a further embodiment, the TaqMan probe is labeled at the 5 'end with a fluorescent reporter group, such as FAM, VIC, etc., and at the 3' end with a fluorescent quencher group, such as TAMRA, etc.
In one embodiment, the kit of the invention further comprises a 2 × PCR master Mix, a positive control, and a 10 × PCR colony enhancer. In one embodiment, the positive control comprises the nucleotide sequence shown in SEQ ID No.5 or SEQ ID No. 7. Preferably, the positive control is the nucleotide sequence shown in SEQ ID NO.5 or SEQ ID NO. 7.
In a fourth aspect, the invention provides a method for detecting Aeromonas veronii using any of the primer pairs, reagents or kits described herein. Alternatively, a fourth aspect of the invention provides the use of any primer pair, reagent or kit of the invention in the preparation of a detection agent for detecting aeromonas veronii.
In one embodiment, detecting aeromonas veronii comprises the steps of:
a. taking the genome DNA or a single colony of a sample to be detected as a PCR template, performing PCR amplification by using a primer, and determining that an amplification product is positive after electrophoresis analysis and has the same band with a positive control, wherein the positive control is a nucleotide sequence shown in SEQ ID NO.5 or SEQ ID NO. 7.
In a further embodiment, the above-described method of the present invention further comprises the steps of:
b. recovering positive amplification products, carrying out sequencing analysis, and comparing with a sequence shown in SEQ ID NO.5 or SEQ ID NO. 7; and
c. based on the alignment results, a test sample having a sequence homology of 99% or more (e.g., 99%, 99.5%, 100%, or any value therebetween) is determined to be positive for Aeromonas veronii, i.e., the presence of Aeromonas veronii is detected.
In a further embodiment, the PCR reaction system in step a is:
sample DNA to be tested (200 ng/ul): 1 mul;
forward and reverse primers (10. mu.M): 1 μ l each;
2×PCR master Mix:25μl;
double water distillation: 22 mu l of the solution;
a total of 50. mu.l was obtained.
In a further embodiment, the positive control is a positive control comprising or consisting of the nucleic acid sequence shown in SEQ ID No.5 or SEQ ID No.7 or the positive control is an identified wild-type aeromonas veronii.
In a further embodiment, wherein the PCR amplification procedure in step a is:
pre-denaturation at 94 ℃ for 5 min;
denaturation at 94 ℃ for 30 s;
annealing at 58 ℃ for 30 s;
extension at 72 ℃ for 30 s;
a total of 25 cycles;
extension was continued for 7min at 72 ℃.
In one embodiment, the method or use of the invention is used for detecting the presence of aeromonas veronii in human, mouse, livestock and poultry, arthropod, reptile (such as eriocheir sinensis, Chinese softshell turtle and the like), aquatic animal and other species, especially aquatic animal and other species (such as tilapia, loach, koi, channel catfish and the like), and particularly for detecting the presence of aeromonas veronii in a bacterial mixture.
In a further embodiment, the method or use of the invention is for detecting one or more of aeromonas veronii strain B565, AVNIH1, TH0426 or CB 51. Preferably, the method or use of the invention is for detecting aeromonas veronii strain B565.
A fifth aspect of the present invention provides a method for developing a primer for detecting Aeromonas veronii, the method comprising the steps of:
1) analyzing all protein sequences included in NCBI by writing python program script by bioinformatics means, thereby obtaining aeromonas veronii specific nucleotide sequences;
2) respectively designing at least one pair of primers aiming at each section of specific sequence based on the specific nucleotide sequence of the Aeromonas veronii obtained in the step 1); and
3) carrying out PCR amplification on the genomic DNA of the Aeromonas veronii by using the primers designed in the step 2), and screening out the primers capable of specifically amplifying the specific sequence of the Aeromonas veronii.
In one embodiment, the method further comprises step 4): the nucleic acid sequence of the target PCR product is determined by sequencing.
In one embodiment, the above step 1) includes the following steps (refer to fig. 1):
(a) obtaining a data subset 1 and a data subset 2 from the NCBI database, wherein the data subset 1 includes all protein sequences of aeromonas (level of genus) but does not include any protein sequence of aeromonas veronii (level of species) included in the NCBI database, and the data subset 2 includes all protein sequences of aeromonas veronii (level of species) included in the NCBI database; and performing Blast alignment on the sequences in the data subset 1 and the data subset 2 to obtain a sequence subset a and a sequence subset a (which is equivalent to screening a species-specific protein sequence at the genus level), wherein the sequence subset a is composed of the sequences in the data subset 2 which can not be matched with the data subset 1, and the sequence subset a is composed of the sequences in the data subset 2 which can be matched with the data subset 1;
(b) obtaining a data subset 3 from the NCBI database, wherein said data subset 3 comprises protein sequences of all species included in the NCBI database, but does not comprise any protein sequences of the genus aeromonas veronii (level of genus); and performing Blast alignment on the sequence subset A and the sequences in the data subset 3 to obtain a sequence subset B and a sequence subset B (which is equivalent to screening specific protein sequences of Aeromonas veronii species at the level of all species), wherein the sequence subset B consists of the sequences in the sequence subset A which cannot be matched with the data subset 3, and the sequence subset B consists of the sequences in the sequence subset A which can be matched with the data subset 3;
(c1) when the number of sequences in the sequence subset B is not zero, converting the sequences in the sequence subset B into nucleic acid sequences, thereby generating a sequence subset B ', and performing Blast alignment of all nucleic acid sequences in the sequence subset B' with nucleic acid sequences of all species included in the NCBI database (which is equivalent to screening of nucleic acid sequences specific to the species of aeromonas veronii at the species level), thereby screening of protein sequences X1 specific to aeromonas veronii (at the species level); or
(c2) When the number of sequences in sequence subset B is zero, then obtaining a data subset 4 from the NCBI database, said data subset 4 comprising all protein sequences of the family aeromonas (level of family) as included in the NCBI database, but not including any protein sequences of the genus aeromonas vickers (level of genus); and performing Blast alignment on the sequence subset a and the sequences in the data subset 3 to obtain a sequence subset C and a sequence subset C (which is equivalent to screening specific protein sequences of Aeromonas veronii at the family level), wherein the sequence subset C consists of the sequences in the sequence subset a which can not be matched with the data subset 4, and the sequence subset C consists of the sequences in the sequence subset a which can be matched with the data subset 4;
(d2) obtaining a data subset 5 from the NCBI database, wherein said data subset 5 comprises protein sequences of all species included in the NCBI database, but does not comprise any protein sequences of the family aeromonas veronii (level of family); and performing Blast alignment on the sequence subset C with the sequences in the data subset 5, thereby obtaining a sequence subset D and a sequence subset D (which is equivalent to screening specific protein sequences of Aeromonas veronii at the level of all species), wherein the sequence subset D consists of the sequences in the sequence subset C which cannot be matched with the data subset 5, and the sequence subset D consists of the sequences in the sequence subset C which can be matched with the data subset 5;
(e2) when the number of sequences in the sequence subset D is not zero, converting the sequences in the sequence subset D into nucleic acid sequences, thereby generating a sequence subset D ', and performing Blast alignment of all nucleic acid sequences in the sequence subset D' with nucleic acid sequences of all species included in the NCBI database (which is equivalent to screening of nucleic acid sequences specific to the species of aeromonas veronii at the genus level), thereby screening for an aeromonas veronii-specific protein sequence X2; or
(e3) When the number of sequences in the sequence subset D is zero, a third round is entered, and corresponding data subsets are set according to the aforementioned concept, and specific protein sequences of the family of the objective horizontal screening, specific proteins of the objective at the class level, specific protein sequences of the class at the phylum level are sequentially started, and further screening is performed at the level of all species, and finally, family, order, class, or phylum specific protein sequences X3, X4, X5, or X6 are screened.
Through the complete circulation, the best condition is that a protein sequence X1 with specificity of Aeromonas veronii species can be screened out through the first circulation; the most complicated case is that six segments of X1-X6 representing different classification levels are screened after six cycles of species, genus, family, order, class and phylum, and the common combination is used for identifying the existence of Aeromonas veronii. In the present invention, the inventors fortunately screened for protein sequence X1 specific for the A.victoriae species by the first round of cycling.
In one embodiment, the step 1) further comprises performing TBLASTn (protein → nucleotide, i.e., translation of the nucleic acid sequence in the library into a protein sequence, and then performing protein-to-protein alignment with the sequence to be searched) alignment of the obtained protein sequence specific to aeromonas veronii (species level) with the sequences in the NCBI nucleic acid database, thereby further determining that the obtained protein sequence is specifically present in aeromonas veronii. Further, the step 1) further comprises selecting a nucleic acid sequence with 100% matching degree obtained by Blast detection as a nucleic acid sequence specific to Aeromonas veronii (species level).
In one embodiment, step 2) above includes Primer design using Primer Premier 5.0 and DNAMAN software.
In one embodiment, the PCR reaction system in step 3) above further comprises genomic DNA of other bacteria as a negative control. Further, the other bacteria are selected from Bacillus subtilis (Bacillus subtilis), Vibrio parahaemolyticus (Vibrio parahaemolyticus), Edwardsiella tarda (Edwardsiella tarda), Vibrio alginolyticus (Vibrio alginolyticus), Escherichia coli (Escherichia coli), Pseudomonas aeruginosa (Pseudomonas aeruginosa), or any combination thereof.
In a preferred embodiment, the method of the invention screens for a protein sequence specific to Aeromonas veronii (species level) as shown in SEQ ID No.6 or a nucleic acid sequence specific to Aeromonas veronii (species level) as shown in SEQ ID No.5, the protein and nucleic acid sequence characteristics being as shown in Table 1 below.
TABLE 1 characteristics of Aeromonas veronii-specific proteins and their corresponding nucleic acid sequences
Figure BDA0001632633840000091
Figure BDA0001632633840000101
More preferably, the method of the present invention obtains primer sequences represented by SEQ ID NO.1-4, and the primer sequence information is shown in Table 2 below.
TABLE 2 primer sequence information shown by SEQ ID NO.1-4
Figure BDA0001632633840000102
In one embodiment, the product of the PCR reaction performed by the primers WP _041202667.1F and WP _041202667.1R has the nucleic acid sequence shown in SEQ ID NO. 5; the product obtained by PCR reaction of the primers WP _041202667.1_ part F and WP _041202667.1_ part R has the nucleic acid sequence shown in SEQ ID NO. 7.
In the present invention, the terms "primer" and "primer pair" are used interchangeably unless the context indicates otherwise. The terms "Vibrio" and "Aeromonas veronii" are used interchangeably and refer to the bacteria Aeromonas veronii, Latin under the name Aeromonas veronii.
The foregoing is illustrative only and is not intended to be limiting in any way. In addition to the illustrative aspects, embodiments, and features described above, further aspects, embodiments, and features will be more readily understood by reference to the following detailed description.
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Further aspects, features of the present invention will be more readily understood by reference to the following drawings. It will be appreciated by persons skilled in the art that these drawings illustrate only some embodiments according to the invention, and should not be taken as limiting the scope of the invention.
FIG. 1 shows a logical diagram for finding species-specific sequences of Aeromonas veronii.
FIG. 2 shows the results of TBLASTn alignment of the protein sequence SEQ ID NO.6 specific to Aeromonas veronii (species level) obtained according to the invention in the NCBI nucleic acid database.
Fig. 3 shows the specific PCR detection results of WP _041202667.1_ par primer pair, where M: DNA marker DL 2000; 1: wild type aeromonas veronii; 2-7: an Aeromonas veronii tmRNA gene knockout strain.
Fig. 4 shows the specific PCR detection results of WP _041202667.1_ part primer pair, where M: DNA marker DL 2000; 1: b, bacillus subtilis; 2: vibrio parahaemolyticus; 3: wm3064 E.coli; 4: wild type vitamin bacteria; 5-6: an Aeromonas veronii tmRNA gene knockout strain.
Fig. 5A shows the specific PCR detection results for the WP _041202667.1 primer pair, where M: DNAmarker DL 2000; 1: b, bacillus subtilis; 2: vibrio parahaemolyticus; 3: aeromonas veronii; 4: edwardsiella tarda; 5: vibrio alginolyticus; 6: e.coli; 7: pseudomonas aeruginosa.
Fig. 5B shows the results of specific PCR detection of the 16s rDNA universal primer pair, where M: DNAmarker DL 2000; 1: b, bacillus subtilis; 2: vibrio parahaemolyticus; 3: aeromonas veronii; 4: edwardsiella tarda; 5: vibrio alginolyticus; 6: e.coli; 7: pseudomonas aeruginosa.
Detailed Description
In the following, only certain exemplary embodiments are briefly described. As those skilled in the art will recognize, the described embodiments may be modified in various different ways, all without departing from the spirit or scope of the present invention. Accordingly, the drawings and description are to be regarded as illustrative in nature, and not as restrictive.
Unless otherwise specified, the technical means used in the examples are conventional means well known to those skilled in the art; all reagents used in the examples are commercially available unless otherwise specified.
Example 1 mining of specific sequences at the Aeromonas veronii species level
All protein sequences included in NCBI were analyzed by writing a python program script using bioinformatics approach, according to the flow shown in fig. 1.
The process shown in FIG. 1 comprises the following steps:
(a) obtaining a data subset 1 and a data subset 2 from the NCBI database, wherein the data subset 1 includes all protein sequences of aeromonas (level of genus) but does not include any protein sequence of aeromonas veronii (level of species) included in the NCBI database, and the data subset 2 includes all protein sequences of aeromonas veronii (level of species) included in the NCBI database; and performing Blast alignment on the sequences in the data subset 1 and the data subset 2 to obtain a sequence subset a and a sequence subset a (which is equivalent to screening a species-specific protein sequence at the genus level), wherein the sequence subset a is composed of the sequences in the data subset 2 which can not be matched with the data subset 1, and the sequence subset a is composed of the sequences in the data subset 2 which can be matched with the data subset 1;
(b) obtaining a data subset 3 from the NCBI database, wherein said data subset 3 comprises protein sequences of all species included in the NCBI database, but does not comprise any protein sequences of the genus aeromonas veronii (level of genus); and performing Blast alignment on the sequence subset A and the sequences in the data subset 3 to obtain a sequence subset B and a sequence subset B (which is equivalent to screening specific protein sequences of Aeromonas veronii species at the level of all species), wherein the sequence subset B consists of the sequences in the sequence subset A which cannot be matched with the data subset 3, and the sequence subset B consists of the sequences in the sequence subset A which can be matched with the data subset 3;
(c1) when the number of sequences in the sequence subset B is not zero, converting the sequences in the sequence subset B into nucleic acid sequences, thereby generating a sequence subset B ', and performing Blast alignment of all nucleic acid sequences in the sequence subset B' with nucleic acid sequences of all species included in the NCBI database (which is equivalent to screening of nucleic acid sequences specific to the species of aeromonas veronii at the species level), thereby screening of protein sequences X1 specific to aeromonas veronii (at the species level); or
(c2) When the number of sequences in sequence subset B is zero, then obtaining a data subset 4 from the NCBI database, said data subset 4 comprising all protein sequences of the family aeromonas (level of family) as included in the NCBI database, but not including any protein sequences of the genus aeromonas vickers (level of genus); and performing Blast alignment on the sequence subset a and the sequences in the data subset 3 to obtain a sequence subset C and a sequence subset C (which is equivalent to screening specific protein sequences of Aeromonas veronii at the family level), wherein the sequence subset C consists of the sequences in the sequence subset a which can not be matched with the data subset 4, and the sequence subset C consists of the sequences in the sequence subset a which can be matched with the data subset 4;
(d2) obtaining a data subset 5 from the NCBI database, wherein said data subset 5 comprises protein sequences of all species included in the NCBI database, but does not comprise any protein sequences of the family aeromonas veronii (level of family); and performing Blast alignment on the sequence subset C with the sequences in the data subset 5, thereby obtaining a sequence subset D and a sequence subset D (which is equivalent to screening specific protein sequences of Aeromonas veronii at the level of all species), wherein the sequence subset D consists of the sequences in the sequence subset C which cannot be matched with the data subset 5, and the sequence subset D consists of the sequences in the sequence subset C which can be matched with the data subset 5;
(e2) when the number of sequences in the sequence subset D is not zero, converting the sequences in the sequence subset D into nucleic acid sequences, thereby generating a sequence subset D ', and performing Blast alignment of all nucleic acid sequences in the sequence subset D' with nucleic acid sequences of all species included in the NCBI database (which is equivalent to screening of nucleic acid sequences specific to the species of aeromonas veronii at the genus level), thereby screening for an aeromonas veronii-specific protein sequence X2; or (e3) when the number of sequences in the sequence subset D is zero, entering a third round, setting corresponding data subsets according to the aforementioned thought, and starting specific protein sequences of the family selected at the target level, specific proteins of the target selected at the class level, specific protein sequences of the class selected at the phylum level, and further selecting at all species levels, finally selecting specific protein sequences of the family, the order, the class, or the phylum X3, X4, X5 or X6.
Through the complete circulation, the best condition is that a protein sequence X1 with specificity of Aeromonas veronii species can be screened out through the first circulation; the most complicated case is that six segments of X1-X6 representing different classification levels are screened after six cycles of species, genus, family, order, class and phylum, and the common combination is used for identifying the existence of Aeromonas veronii.
In this example, the above analysis process only involves steps (a) to (c1) because the selected subset of sequences B contains the protein sequence represented by SEQ ID NO.6, i.e., the number of sequences in subset B is not zero.
And (c) performing TBLASTn comparison on the obtained specific protein sequence of the Aeromonas veronii (species level) in the step (c1) and the sequence in the NCBI nucleic acid database, and further determining that the obtained protein sequence is specifically present in the Aeromonas veronii, wherein the comparison result is shown in FIG. 2. Then, a nucleic acid sequence (shown as SEQ ID NO. 5) with a matching degree of 100% obtained by Blast detection was selected as a nucleic acid sequence specific to Aeromonas veronii (species level). The protein and nucleic acid sequence features are shown in table 1.
Example 2 test materials, test methods and apparatus
1. Test materials and apparatus
The strain is as follows:
bacillus subtilis (Bacillus subtilis), Vibrio parahaemolyticus (Vibrio parahaemolyticus), Aeromonas veronii (Aeromonas veronii), Edwardsiella tarda (Edwardsiella tarda), Vibrio alginolyticus (Vibrio algornyticus), Escherichia coli (Escherichia coli), and Pseudomonas aeruginosa (Pseudomonas aeruginosa) were all stored in the laboratory.
Culture medium and reagents:
the bacterial genome DNA rapid extraction kit (cargo number N1152) and PCR reaction reagents are purchased from Dongshen Biotech, Inc. of Guangzhou (Dongsheng Biotech Co., Ltd., Ltd);
tryptone, yeast extract, agar powder, agarose were purchased from Guangdong Weijia biology, Inc.;
1) LB liquid medium, containing the following: tryptone 1.0g, yeast extract 0.5g, NaCl 0.5g, distilled water 100mL, using 10mol/L NaOH to adjust pH to 7.2, high pressure sterilization at 121 ℃ for 20min, and storing at 4 ℃ for standby.
2) LB solid medium, containing the following: tryptone 1.0g, yeast extract 0.5g, NaCl 0.5g, agarose 1.5g, distilled water 100mL, using 10mol/L NaOH to adjust pH to 7.2, high pressure sterilization at 121 ℃ for 20min, cooling to about 50 ℃ and pouring into a flat plate, preserving for later use.
3)100mg/ml Amp (ampicillin)
Amp 100mg, dissolved in 1ml of sterile water, filter sterilized with a filter of 0.22 μm diameter, and stored at-20 ℃.
4)25mg/ml Cam (kanamycin)
Cam 50mg was dissolved in 2ml of an absolute ethanol solution and divided into 0.5ml portions and stored at-20 ℃.
5) Agarose gel electrophoresis reagent
50 × TAE buffer: tris base 242g, Na2EDTA·2H2O37.2 g and glacial acetic acid 57.1ml, and deionized water was added thereto to dissolve the mixture sufficiently to 1000ml, followed by storage at room temperature.
6) 1% agarose solution: 0.2g of agarose was weighed, added to 20ml of TAE buffer, and dissolved by heating.
Instrumentation and equipment
QYC-2102C Total temperature shaking culture bed purchased from instrument Limited of New Jiangnan of science and technology park of Ningbo city; the HH-2 digital display constant temperature water bath kettle is purchased from China electric appliance, Inc. of Changzhou China; the LDZX-50KB vertical pressure steam sterilizer is purchased from Shanghai Shenan medical instrument factory; the HPX-9272MBE digital display electric heating incubator is purchased from Shanghai Boxun industry Co., Ltd; the WH-861 vortex mixer is purchased from Hualida experimental equipment, Inc. of Taicang city, and the SW-CJ-2D double single-face purification workbench is purchased from Suzhou purification equipment, Inc.; centrifuge5417R desk-top high speed Centrifuge was purchased from Eppendorf, germany; the Nanodrop2000 nucleic acid protein detector was purchased from Thermo corporation, usa; CP214 electronic balance purchased from aohaus instruments (shanghai) ltd; AG22331Hamburg type PCR amplification instrument was purchased from Eppendorf, Germany; the 1600R full-automatic digital gel imaging analysis system is purchased from Shanghai Tianneng technology, Inc.
2. Test method
(1) Genomic DNA template extraction
The genomic DNA of all strains was extracted using the bacterial genomic DNA rapid extraction kit (cat # N1152) according to the instructions. The DNA mass was determined by agarose gel and the concentration of DNA was determined using a Nanodrop2000 nucleic acid protein detector.
(2) Colony PCR template preparation
Scraping a small amount of bacterial colony, adding 100uL of sterile water, blowing and beating into uniform bacterial liquid by a pipette, carrying out boiling water bath for 5min, then centrifuging at 12,000rpm for 1min, and taking supernatant as a bacterial colony PCR template.
(3) PCR amplification of specific fragment products
Using bacterial genome DNA or single colony crude extract as template, and respectively amplifying specific sequence products by using primers.
Taking 5 mul PCR amplification product, using 30g/L agarose gel for electrophoresis separation, using DNA marker DL2000 as molecular weight marker, voltage is 5V/cm, after electrophoresis for 20min, using gel image scanner for analysis and photograph.
(4) PCR reaction system and reaction procedure.
PCR reaction (50. mu.l):
Figure BDA0001632633840000161
PCR reaction procedure: 25 cycles
Figure BDA0001632633840000162
Example 3 primer design and primer screening based on Aeromonas veronii species level specific sequences
Using Primer Premier 5.0 and DNAMAN software, a plurality of sets of primers were designed for the specific nucleic acid sequences obtained in example 1, and the designed primers were synthesized by Shanghai Biometrics Ltd.
PCR was carried out by the method of example 2 using Aeromonas veronii genomic DNA as a template and different primer pairs designed and synthesized. The PCR amplification products were analyzed by 30g/L agarose gel electrophoresis.
Based on the results of gel electrophoresis (not shown), a single primer pair with a clear amplified band was selected for further primer specificity analysis. Two pairs of primers are obtained, the sequences of the primers are shown by SEQ ID No.1-4, and the sequence information of the primers is shown in Table 2. The amplified product is further sequenced to confirm that the target fragment is consistent with the sequence shown in SEQ ID NO.5 or SEQ ID NO. 7.
Example 4 verification of Aeromonas veronii specific primers
Using the primer pairs obtained in example 3, PCR reactions were carried out using genomic DNAs of Bacillus subtilis, Vibrio parahaemolyticus, Aeromonas veronii wild-type and tmRNA gene-deleted strains, Edwardsiella tarda, Vibrio alginolyticus, Escherichia coli, and Pseudomonas aeruginosa as templates, respectively, according to the method of example 2. The PCR amplification products were analyzed by 30g/L agarose gel electrophoresis.
Gel electrophoresis results (fig. 3,4 and 5A) show that the primer pair of the invention can amplify fragments with expected sizes for both wild type and specific gene-deleted strains of aeromonas veronii, and can only amplify target fragments in aeromonas veronii, and target fragments cannot be obtained in other negative control strains. As an internal control, 16s rDNA universal primer pairs SEQ ID NO.8 and SEQ ID NO.9 were used, and PCR amplification was performed using the same genomic DNA as described above, and products having the same size and concentration were obtained in each sample, further demonstrating that the primer pair of the present invention has specificity for Aeromonas veronii (FIG. 5B).
And further sequencing the amplified fragment, and determining that the amplified fragment is a specific nucleic acid sequence of the aeromonas veronii through sequence comparison analysis.
The above description is only for the specific embodiment of the present invention, but the scope of the present invention is not limited thereto, and any person skilled in the art can easily conceive various changes or substitutions within the technical scope of the present invention, and these should be covered by the scope of the present invention. Therefore, the protection scope of the present invention shall be subject to the protection scope of the appended claims.
Sequence listing
<110> university of Hainan
<120> Aeromonas veronii detection primers, kit, detection method and development method thereof based on specific sequence
<141> 2018-1-8
<160> 9
<170> SIPOSequenceListing 1.0
<210> 1
<211> 22
<212> DNA
<213> Artificial sequence (Artificial sequence)
<400> 1
aacatcatgg tgccgccaac gt 22
<210> 2
<211> 22
<212> DNA
<213> Artificial sequence (Artificial sequence)
<400> 2
atggtcgcag agcttgtcat ct 22
<210> 3
<211> 21
<212> DNA
<213> Artificial sequence (Artificial sequence)
<400> 3
cagcacaata gaacaccaga c 21
<210> 4
<211> 18
<212> DNA
<213> Artificial sequence (Artificial sequence)
<400> 4
atggtcgcag agcttgtc 18
<210> 5
<211> 192
<212> DNA
<213> Aeromonas veroni (Ameromonas veronii)
<400> 5
aacatcatgg tgccgccaac gtgcgcagca caatagaaca ccagacatcc gatacccgac 60
caagtcagga aatagggtga taaaacgagc gagcccaatg gcggatattt gggtgatcag 120
cagtaataac gatgcgatga tctctccccc ttcggggaaa taacagagcc agatgacaag 180
ctctgcgacc at 192
<210> 6
<211> 64
<212> PRT
<213> Aeromonas veroni (Ameromonas veronii)
<400> 6
Met Val Ala Glu Leu Val Ile Trp Leu Cys Tyr Phe Pro Glu Gly Gly
1 5 10 15
Glu Ile Ile Ala Ser Leu Leu Leu Leu Ile Thr Gln Ile Ser Ala Ile
20 25 30
Gly Leu Ala Arg Phe Ile Thr Leu Phe Pro Asp Leu Val Gly Tyr Arg
35 40 45
Met Ser Gly Val Leu Leu Cys Cys Ala Arg Trp Arg His His Asp Val
50 55 60
<210> 7
<211> 167
<212> DNA
<213> Aeromonas veroni (Ameromonas veronii)
<400> 7
cagcacaata gaacaccaga catccgatac ccgaccaagt caggaaatag ggtgataaaa 60
cgagcgagcc caatggcgga tatttgggtg atcagcagta ataacgatgc gatgatctct 120
cccccttcgg ggaaataaca gagccagatg acaagctctg cgaccat 167
<210> 8
<211> 20
<212> DNA
<213> Artificial sequence (Artificial sequence)
<400> 8
agagtttgat catggctcag 20
<210> 9
<211> 22
<212> DNA
<213> Artificial sequence (Artificial sequence)
<400> 9
tagggttacc ttgttacgac tt 22

Claims (4)

1. Use of a primer pair for the preparation of a detection agent for detecting Aeromonas veronii, wherein:
(1) the nucleotide sequence of the forward primer of the primer pair is selected from one or more of the following: the nucleotide sequence shown in SEQ ID NO.1 and the nucleotide sequence shown in SEQ ID NO. 3; and
(2) the nucleotide sequence of the reverse primer of the primer pair is selected from one or more of the following: the nucleotide sequence shown in SEQ ID NO.2 and the nucleotide sequence shown in SEQ ID NO. 4.
2. The use of claim 1, wherein one primer of the primer pair is detectably labeled.
3. The use as claimed in claim 2, wherein the label is selected from the group consisting of a radioisotope, an enzyme, a fluorescent substance, a luminescent substance or biotin.
4. The use according to any one of claims 1 to 3, wherein:
the primer pair is a primer pair WP _041202667.1, the nucleotide sequence of a forward primer is shown as SEQ ID NO.1, and the nucleotide sequence of a reverse primer is shown as SEQ ID NO. 2; or
The primer pair is a primer pair WP _041202667.1_ par, the nucleotide sequence of the forward primer is shown as SEQ ID NO.3, and the nucleotide sequence of the reverse primer is shown as SEQ ID NO. 4.
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副溶血弧菌高通量分子检测方法的建立与基因分型研究;陈万义;《中国博士学位论文全文数据库 医药卫生科技辑》;20111215;正文第2.1.5节,图2-1 *

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