CN107365840B - Cervidae animal rapid identification kit based on DNA bar code and application thereof - Google Patents

Cervidae animal rapid identification kit based on DNA bar code and application thereof Download PDF

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CN107365840B
CN107365840B CN201710551525.8A CN201710551525A CN107365840B CN 107365840 B CN107365840 B CN 107365840B CN 201710551525 A CN201710551525 A CN 201710551525A CN 107365840 B CN107365840 B CN 107365840B
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陈星�
白加德
宣晶
孟玉萍
钟震宇
单云芳
程志斌
王丽斌
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Beijing Milu Ecological Experiment Center
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Abstract

The invention provides a rapid Cervidae animal identification kit based on DNA bar codes and application thereof. The cervidae animal identification kit of the present invention includes one or more of the following labeled or unlabeled DNA sequences or barcodes thereof: SEQ ID No.5, SEQ ID No.6, SEQ ID No.7, SEQ ID No. 8. The kit can rapidly identify the cervidae animals and species.

Description

Cervidae animal rapid identification kit based on DNA bar code and application thereof
Technical Field
The invention relates to a cervidae animal identification kit and application thereof, in particular to a cervidae animal rapid identification kit based on a DNA bar code and application thereof.
Background
The DNA Barcoding (DNA Barcoding) technique is a new method of biological classification, which is a product of a combination of molecular biology and bioinformatics. This concept assumes that every organism on earth can be identified by rapid analysis of a small piece of its DNA. In recent years, this technology has become a hot spot of research in the biology taxonomy, and has an important role in the identification of the biology taxonomy, and the mitochondrial cytochrome C oxidase I subunit (mtCOI) has been widely used as a recommended sequence of DNA barcode in the animal kingdom in different researchers and research groups.
In 2009, with the development of DNA extraction technology, PCR technology, and high-throughput sequencing technology, especially the popularization and application of DNA barcode technology, it was widely accepted that mitochondrial COI genes, which are the first choice for DNA barcode technology, are widely used in domestic research on cervidae animals.
In the genetic relationship research of cervidae animals, the ceriphora chinensis (2009) carries out DNA barcode research on 16 rare endangered wild animals in China, and the DNA barcode research ranges from cervidae, mustaceae, bovidae, Camelidae (Camelidae) and equines (Equidae), and totally belongs to 15 genera. Based on the sequence analysis of two sections of COI with 655bp and 404bp, the phylogenetic relationship between the deer and other closely sourced species is discussed.
In the aspect of rapid identification of medicinal materials, the COI gene is used as a recommended sequence of a DNA bar code and is also widely applied to deer animals such as antler decoction pieces (ZhangRong, etc., 2011; trelina, etc., 2012) and traditional Chinese medicinal materials (Liudong, etc., 2014) of deer animals.
In addition, the cervids and related products have a wide application market as trade products, wherein the traditional method is difficult to distinguish or needs long-term professional training without various adulterants, so that the DNA barcode technology capable of performing rapid identification is widely applied to such research (Cai et al, 2015; Luo et al, 2013).
After new technologies such as protein analysis, PCR technology, DNA sequencing technology and the like appear, the rapid development of molecular systematics and DNA molecular technology brings questions to the original morphological theory. Emerson & Tate (1993) analyzed the evolutionary relationships of 10 species and subspecies of 4 genera of the subfamily cervidae by protein electrophoresis, suggesting a new view that they thought that elk (Elaphurus) is more closely related to cervi (Cervus), while water deer (C. unicolor) in cervi is more closely related to fallow deer (Dama) and spotted deer (Axis) than to other species of cervi. Randi et al (2001) investigated phylogenetic relationships of 25 species and subspecies of the subfamily Cervinae (Cervinae) and Muntiacae (Muntiacinae) based on the complete sequence analysis of D-loop of mtDNA. Polziehn & Strobeck (2002) phylogenetically analyzed various subspecies of red deer (C.elaphus) established in the traditional classification based on the DNA sequence of mtDNA control region, and it was considered that the red deer in the traditional classification is not a monophyletic group and should be classified into red deer (C.elaphus) mainly distributed in Europe, North Africa to Central Asia and red deer (Canada red deer) distributed in North America and east Asia and Siberian, which has only one subspecies of red deer (C.elaphus yarkandensis) in China. Hassanin et al (2012) performed full-length sequencing on 210 mtDNAs of a species of the order Cetartiodactyla, including 107 species 183, and reconstructed phylogenetic trees of the species of the order Cetartiodactyla based on the full-length sequences of the mtDNAs, clarified evolutionary divergence events, and estimated evolution time by molecular clock correction. The results show that the deer family has a close relationship with the mustaceae (Moschidae) and Bovidae (Bovidae), the branch is separated from the order cetacea and artiodae from late-to-early-new-age, and the mustaceae has a close relationship with the cattle family, and is different from the traditional taxonomy point of view, and the mustaceae is considered to be differentiated later than the deer family and belongs to a more evolved group.
Early domestic studies on molecular levels of cervidae animals have mainly focused on cytochrome b gene (cytb) fragments of mitochondrial DNA, as in plum et al (1999) discussed phylogenetic relationships of cervidae animals from four species of cervidae animals, such as buffalo deer, sika deer and red deer: cytochrome b gene segments of mitochondrial DNA are respectively amplified, and a 367bp base sequence is obtained through determination, and the sequence difference between the cytochrome b gene segments and the base sequence is 4.09-7.08%. The construction and analysis of the molecular system evolution tree are carried out by using an NJ method, a maximum reduction method and a maximum likelihood method, and the method is obtained, wherein the Cervus elaphus, the Cervus nippon Temminck, and the Cervus Elaphus are differentiated about 240-280 ten thousand years ago, and the Cervus elaphus and the Cervus Elaphus are differentiated about 160 ten thousand years ago. In 2003, Liu Zhu Hua, etc. have discussed the evolutionary relationship among the subfamily Cervidae, genus Cervus, and subfamily Cervus elaphus according to the sequence analysis of cytb gene. Analysis of the results shows that: in current classification systems, the genus cervus may not occur unilineage, suggesting that ragdeer should be incorporated into the genus cervus; elk has a relatively recent evolutionary relationship with the genus cervi, and the genus cervi should also be incorporated; the evolutionary position of the deer in the fallow period is to be further researched; the merged genus cervi is unilineage generation. The species of Cervus elaphus of China are phylogenetically a single group, wherein the species of Cervus elaphus Tianshan and the species of Altai are gathered into the most primitive one.
Database query results by 2013, 9, 1 and show that the amount of DNA barcode sample data of the deer animals is greatly increased. There are 421 effective DNA barcode information (containing 3 species of cytb sequence information) of 55 species of Cervidae (species, subspecies, including partial synonyms), wherein there are 173 effective DNA barcode information (COI sequence is greater than 500bp) in total of 32 species (species, subspecies, including partial synonyms) of Cervidae 9.
The phenomenon that the amplification of the COI gene is difficult in the deer is shown in a general primer, and the amplification is described in many documents (Lianhong, 2009; Zhangni et al, 2011), no deer specific primer exists, and no related kit is applied.
Disclosure of Invention
The invention aims to provide a rapid Cervidae animal identification kit based on DNA bar codes.
In order to achieve the above purpose, firstly, the invention designs a specific primer for the research of DNA bar codes of deer animals and the rapid identification of species. It includes:
SEQ ID No.1(5’-3’):TATTTGGTGCCTGAGCAGGCATAGTCGGAACAGCC;
SEQ ID No.2(5’-3’):GGTGACCAAAGAATCAGAACAAGTGTTGATA。
the specific primer pair is based on the mitochondrial DNA full-length sequence of red deer (Cervus elaphus) (NC _007704) and Cervus nippon (NC _006993) published by Genbank and the related sequence summary design of a plurality of different species such as fragment sequence information (KF509972, KF5099733) of COI genes of elk (Elaphurus davidianum), can be used for amplifying different deer animals, has better specificity and good amplification effect, and well solves the problems of difficult amplification and easy obtaining of wrong sequence information in the similar research. The length of the amplified fragment is about 600bp, and the application of DNA barcode research can be supported. Thus, the invention further provides a rapid Cervidae animal identification kit based on the DNA barcode.
Specifically, the invention provides a deer animal identification kit, which comprises one or more of the following labeled or unlabeled DNA sequences or barcodes thereof:
SEQ ID No.5, SEQ ID No.6, SEQ ID No.7, SEQ ID No. 8. See below and sequence listing for each specific sequence.
According to the specific embodiment of the present invention, the sequence of imaged barcodes can be seen in fig. 3, 4, 5 and 6. The kit of the invention may comprise one or more of the barcodes as shown in figure 3, figure 4, figure 5 and figure 6.
According to a particular embodiment of the invention, the kit of the invention may further comprise the following cervidae-specific primers:
SEQ ID No.1(5’-3’):TATTTGGTGCCTGAGCAGGCATAGTCGGAACAGCC;
SEQ ID No.2(5’-3’):GGTGACCAAAGAATCAGAACAAGTGTTGATA。
according to a particular embodiment of the invention, the kit of the invention, which may further comprise a molecular systems tree. The molecular system tree is a molecular system tree of a cervidae animal species constructed on the basis of the specific primer and/or the target sequence of the primer. In one embodiment of the present invention, the molecular phylogenetic tree is set up as shown in FIG. 2.
It is understood that the kit may further include a buffer for amplifying a sample, a Taq polymerase, and the like, which are conventional reagents.
The invention also provides application of the kit in identification of the deer species.
In a specific embodiment of the invention, the sequence shown in SEQ ID No.5 is elk-specific. The kit of the present invention includes an imaged barcode of the sequence shown in SEQ ID No.5, and is used to identify the presence or absence of elk components in a sample to be tested.
In another specific embodiment of the invention, the sequence shown in SEQ ID No.6 is specific for Cervus Nippon Temminck. The kit comprises an imaging bar code of a sequence shown in SEQ ID No.6, and is used for identifying whether the sika deer component exists in a sample to be detected.
In another embodiment of the invention, the sequence shown in SEQ ID No.7 is specific for Cervus elaphus. The kit comprises an imaging bar code of a sequence shown in SEQ ID No.7, and is used for identifying whether a red deer component exists in a sample to be detected.
In another specific embodiment of the invention, the sequence shown in SEQ ID No.8 is specific for fallow deer. The kit comprises an imaged bar code of a sequence shown in SEQ ID No.8, and is used for identifying whether the fallow deer component exists in a sample to be detected.
According to a specific embodiment of the present invention, the sample to be tested is a medicinal material (such as deer horn, blood or tissue), a Chinese medicinal preparation (herbal pieces), or a fossil material, which is required to identify whether the deer component is contained and/or the species of the deer is contained.
The technology of the invention has particularly important significance in the following fields:
(1) obtaining specific DNA markers for elk
Elk (elaphus davidianus) is one of the unique genuine deer subfamily animals in China, and because of its special morphological characteristics, it is classified as a single species animal juxtaposed to the genus cervi (Cervus) in the current classification system, and since studies on molecular markers of proteins and nucleic acids of elk and other genus cervi in the later stage have shown that the relationship of the genus elk and the genus cervi is closer in evolutionary relationship, it is suggested to incorporate the genus elk into the genus cervi (Emerson & Tate, 1993; liu hua, 2003). Elk is a special species in China, because of human hunting and environment change, elk is out of place in the Chinese country in 1900 years, then is exported overseas, reintroduced and other items, and is reproduced to more than 2000 in China so far, and elk necessarily has its own characteristics in gene preservation and population reproduction. The technology of the invention can obtain the specific DNA mark of elk, further develop the research of elk historical evolution and genetic relationship, research the evolution law and better promote the development of elk protection business.
(2) Providing molecular level evidence for phylogenetic evolution of Cervidae animals in China
There are 4 genera of Cervus subfamily worldwide, and there are doubts about phylogenetic relationships between and within each genus, particularly within the genus Cervus (Liu Hua et al, 2003). Chinese genus cervi animals include five species, i.e., water deer (Cervus unicolor), deer antlers (c.edli), white-lipped deer (c.albicostatsis), sika deer (c.nippon) and red deer (c.elaphus). Since the deer animal represents the evolution process of its phylogenetic stage species in the modern species (Floripav, 1957), it is a good material for the evolution form and evolution process research in chemical research. China is the evolution stage of the deer animals, and the development and evolution stages of various species and various subspecies are distributed throughout China (1992, Theassian), so that the method has important theoretical significance for the systematic evolution research of the deer animals in China. Due to the special status of Chinese deer animals, great interest has been raised by many scholars. The invention provides molecular level evidence for systematic evolution research of Cervidae animals in Cervidae from the perspective of molecular biology by taking a specific section of a specific gene, namely mitochondrial cytochrome C oxidase I subunit (mt COI), of Cervidae animals in Cervidae subfamily of China as a research object.
(3) Provides evidence for identifying the material of the bone cultural relics and the geographic distribution of wild species of elk in the ancient period
The unearthed wild elk fossil indicates that elk has originated more than 200 million years ago from today, is most prosperous from about 1 million years ago to about 3000 years from today, the number of elk fossil points or the number of specimens of a certain fossil point in China is extremely rich, elk bones and elk horns are particularly favored by ancient people, and the appearance of cultural relics such as elk bones and the like in the middle of West week is found. However, many deer horns and deer bones are made into products such as cold weapons such as arrow clusters and the like or worn ornaments and the like, and specific types of cultural relics can not be identified due to the change of the shapes. The distribution of these cultural relics provides the most detailed evidence for the geographical distribution of wild species of elk in the ancient period.
(4) The material evidence of criminal cases is judiciously identified, and scientific basis is provided for protecting criminal cases by wild animals
Elk is a national level wild animal protection law which forbids business transaction or eating, and elk DNA molecular marking achievement is adopted to be compared with the material evidence of criminal cases in a molecular mode to identify the material source of the material evidence.
(5) Molecular identification of Chinese medicinal materials, and effective means for circulation and market management of Chinese medicinal materials
The pilose antler, the deer penis, the deer tail, the deer fetus, the deer tendon, the deer bone and the like are the common commercial Chinese medicinal materials in China. But the efficacy of different deer is different, elk nourishes yin, sika deer strengthens yang; even if the medicinal efficacy of the deer species with the same medicinal effect is different, the phenomenon that other animals are used as medicinal materials of the pilose antler and the deer horn for sale due to limited resources and the market is full of the medicine; meanwhile, the phenomenon of synonyms of the same things or synonyms of the same foreign matters in the market brings disorder of the medicinal materials sold in the medicinal material market; in order to improve the yield of the deer antler, part of deer farms are used for hybridizing different deer animal species to bring disorder of species and strains. Molecular identification can be carried out on the deer animal traditional Chinese medicinal materials through the molecular marking achievement of the deer animal DNA, and an effective means is provided for medicinal material circulation and market management.
In summary, the invention designs specific primers of the deer COI gene fragment, screens to obtain the reliable DNA sequence of Chinese deer, prepares the imaging bar code based on the sequence, and the kit of the invention can rapidly identify the deer species.
Drawings
FIGS. 1A and 1B show the results of electrophoresis detection of PCR amplification products using universal primers and the characteristic primers of the present invention. Wherein: lanes 1-25 are elk (elaphus davidianus), lanes 26-40 are sika deer (Cervus nippon), lanes 41-47 are fallow deer (Dama), lanes 48-51 are elk (Cervus elaphus), lane 52 is a negative control, Maker is DL5000marker (TAKARA BIO inc., Japan), and fragment sizes are 5000, 3000, 2000, 1000, 750, 500, 250, 100 in that order.
FIG. 2 is a schematic diagram of a molecular phylogenetic tree of a Cervidae animal constructed based on the Maximum Likelihood Method (Maximum Likelihood Method) using the primers of the present invention.
FIG. 3 is an image of DNA barcodes of elk identified by amplification and screening using primers of the invention.
FIG. 4 is an imaged DNA barcode for identifying sika deer amplified and screened using the primers of the present invention.
FIG. 5 is an imaged DNA barcode for identifying Cervus elaphus obtained by amplification and screening using the primers of the present invention.
Fig. 6 is an imaged DNA barcode identifying fallow deer amplified and screened using the primers of the invention.
Detailed Description
In order that the invention may be more clearly understood, it will now be further described with reference to the following examples and the accompanying drawings. The examples are for illustration only and do not limit the invention in any way.
The experimental methods in the examples, in which specific conditions are not noted, are conventional methods and conventional conditions well known in the art, or conditions as recommended by the manufacturer;
the various chemicals used in the examples are commercially available and the primers used are committed to synthesis.
Example 1 specific primer set for identifying Cervidae animals
Extraction of genomic DNA was carried out according to the method of Sambrook & Russel (2001) or according to the instructions of Tiangen blood genome extraction kit (DP318, Tiangen Biochemical technology (Beijing) Ltd.).
The resulting DNA solution was pipetted 1. mu.l, through a micro-UV spectrophotometer
Figure GDA0002597857590000071
ND-1000(NanoDrop Technologies, Inc., USA) was used for DNA concentration determination and was determined by A260/280The ratio of absorbance of (A) to (B) is used to determine the DNA purity.
The composition and content of the PCR reaction system (50. mu.l) are shown in Table 1.
TABLE 1 PCR reaction System
Reaction components Content (wt.)
Genomic DNA 40ng
Tris-HCl 67mM
(NH4)2SO4 16.6mM
Triton X-100 0.45%
Gelatin 0.2mg/ml
MgCl2 2.5mM
dNTPs 50μM
Primer × 2 0.125μM
Taq enzyme 1U
The PCR reaction was performed on a Bio-Rad My Cycler PCR instrument (Bio-Rad Laboratories, Inc., USA) using the following reaction protocol: pre-denaturation at 94 deg.C for 6min, denaturation at 94 deg.C for 30s, renaturation at 55 deg.C for 30s, and extension at 72 deg.C for 60s for 30 cycles, and final extension at 72 deg.C for 10 min.
The reaction product was mixed with 10. mu.l of Loading buffer, and electrophoresed in 1.5% agarose gel for 30min with a constant voltage power supply of 7V/cm. Dyeing for 1-2 min after electrophoresis, observing in an electrophoresis detector, cutting target fragments, placing in a centrifuge tube, and recovering the kit according to Tiangen agarose gel (DP209, Tiangen Biochemical technology)<Beijing>Co., Ltd.) was performed, and 5. mu.l of the recovered product was electrophoretically detected in a micro ultraviolet spectrophotometer
Figure GDA0002597857590000072
ND-1000(NanoDrop Technologies, Inc., USA) was used for DNA concentration determination by recording A260/280The DNA concentration was calculated.
The results of DNA amplification of the COI gene region using the COI universal primers (Folmer et al, 1994) (Table 2) in this example show that the universal primers LCO1490-HCO2198 are not ideal for deer amplification, especially in the results of electrophoresis of PCR products of elk (Elaphurus davidianus) and fallow deer (Dama dam), but are relatively good when applied to Spotted deer (Cervus nippon) (FIG. 1A).
TABLE 2 COI Universal primers
Primer name Primer sequence (5 '-3')
LCO1490(SEQ ID No.3) GGTCAACAAATCATAAAGATATTGG
HCO2198(SEQ ID No.4) TAAACTTCAGGGTGACCAAAAAATCA
According to the invention, specific primer pairs (table 3, SEQ ID No.1 and SEQ ID No.2) for Cervidae species identification and DNA barcode research are redesigned according to the mitochondrial DNA full-length sequence of Cervus elaphus (Cervus elaphus) (NC _007704) and Cervus nippon (Cervus nippon) (NC _006993) published by Genbank and the fragment sequence information (KF509972, KF5099733) of the COI gene of the Cervus elaphus (Cervus nippon) (NC _006993), PCR amplification tests prove that the new primers have good amplification efficiency and specificity (FIG. 1B), have good amplification effects in tested samples of the Cervus elaphus, the Cervus elaphus and the Cervus nippon, and the length of the amplified fragment is about 600bp, so that the application of the DNA barcode research can be supported. Compared with a COI gene fragment universal primer, the primer with specificity for the deer COI gene fragment designed by the invention has better specificity for the deer, proper length of a product fragment and good amplification efficiency (see an amplification electrophoresis example chart for details), and well solves the problems of difficult amplification and easy obtaining of wrong sequence information in similar research.
TABLE 3 specific primer for deer COI of the present invention
Sequence numbering Sequence (5 '-3')
SEQ ID No.1 TATTTGGTGCCTGAGCAGGCATAGTCGGAACAGCC
SEQ ID No.2 GGTGACCAAAGAATCAGAACAAGTGTTGATA
The specific primer pair of the invention is based on the total length sequence of mitochondrial DNA of red deer (Cervus elaphus) (NC-007704) and sika deer (Cervus nippon) (NC-006993) published by Genbank and the related sequences of a plurality of different species such as fragment sequence information (KF509972, KF5099733) of COI gene of elk (Elaphurus davidianus), can be amplified for different deer animals, and has good amplification effect. The specific primer pair can be used for assisting species identification of related materials (such as deer horns, traditional Chinese medicine decoction pieces, fossil materials and the like) of the cervidae animals.
And (3) sending the purified DNA to a sequencing company (Shanghai Meiji) for sequencing and identification, performing bidirectional sequencing, and obtaining target COI sequence information after comparison and correction. Alignment with elk and other cervid animal sequences known in Genbank confirmed the correctness of the target fragment.
Example 2 construction of molecular phylogenetic Tree Using target sequences of specific primer pairs
The COI gene related sequences of deer (Cervidae) and closely derived mustaceae (Moschidae) and Tragulidae (Tragulidae) species worldwide were obtained from Genbank query (some species have no record of the COI sequence, and the COI full-length sequence was obtained by analyzing the full-length sequence of mitochondrial genome in the gene bank), and there were a total of 52 sequences of 48 taxa (species or subspecies) (table 4). The sequence information was combined with the obtained COI sequence information of 51 elk aster eucervidae species and aligned using software Clustal W and Bioedit, the aligned sequences were exported as fasta (. fas) and nexus (. nex) format files, and the optimal nucleic acid surrogate model was estimated using the software modelest 3.7 test. Using Muscoidae and Tragulidae species as the foreign population, a Maximum Likelihood tree (Maximum Likeliod Method) was constructed by the software MEGA7(Kumar et al, 2016) using the optimal nucleic acid surrogate model calculated by Modlestest 3.7. The systematic tree test adopts a Bootstrap Method (Bootstrap Method), and the Bootstrap support rate of each branch of the systematic tree is calculated after 1000 times of Bootstrap tests. The obtained molecular system tree (figure 2) shows that DNA fragment sequences obtained according to the specific primer pair provided by the research can be well distinguished from different species and can indicate the genetic relationship among the species, the same species is gathered into one branch in the molecular system tree, while the genetic distance among different species is larger, the genetic relationship is obviously distinguished, and the species can be obviously distinguished.
TABLE 4 COI-related Gene sequence information of Cervidae animals and closely related groups on Genbank
Figure GDA0002597857590000091
Figure GDA0002597857590000101
Note: the class labeled "", is the outer class. The column labeled "-" in the disclosure is the research and confirmation of the inventor.
According to the molecular system tree and the sequence comparison result, reliable representative DNA bar code sample data of the deer animals and the closely related species can be obtained by screening. In this example, the reference sequences obtained for elk, sika, fallow deer and elk are as follows:
(1) elaphurus davidianus
DNA sequence (SEQ ID No.5)
TGAGCAGGCATAGTCGGAACAGCCTTAAGCCTACTGATTCGTGCTGAATTAGGTCAACCCGGTACTCTGCTTGGAGATGACCAAATTTATAATGTTATCGTAACCGCACACGCATTCGTAATAATTTTCTTTATAGTTATACCAATTATAATTGGAGGATTTGGTAATTGACTAGTTCCCCTAATAATTGGTGCCCCAGATATAGCATTCCCTCGAATAAACAATATAAGCTTTTGACTCCTCCCTCCCTCTTTCTTACTACTTTTAGCATCATCTATAGTTGAAGCTGGCGCAGGGACAGGCTGAACTGTGTATCCCCCTCTAGCTGGCAACCTAGCTCACGCAGGAGCTTCAGTAGACTTGACTATTTTTTCTTTACATCTGGCAGGTGTCTCTTCAATTCTGGGGGCCATTAACTTTATTACAACAATTATTAATATAAAACCCCCTGCTATATCACAATATCAAACCCCTCTATTTGTGTGATCCGTACTAGTCACTGCTGTACTCCTACTTCTCTCACTCCCTGTACTAGCAGCCGGAATTACAATACTATTAACAGACCGAAACTTAAATACGACCTTTTTTGACCCAGCAGGAGGCGGAG
An imaged Barcode (illuminated Barcode) is shown in fig. 3.
(2) Cervus nippon
DNA sequence (SEQ ID No.6)
TGAGCAGGCATAGTCGGAACAGCCTTAAGCCTACTGATTCGTGCCGAACTGGGCCAACCTGGTACTCTGCTTGGAGATGATCAAATTTATAATGTTATCGTAACCGCACATGCATTCGTAATAATTTTCTTTATAGTTATACCAATTATAATCGGAGGATTTGGTAATTGACTAGTTCCCCTAATAATTGGTGCCCCAGACATAGCATTCCCTCGAATAAACAATATAAGCTTTTGACTCCTCCCTCCTTCTTTCTTACTACTTTTAGCATCATCTATAGTTGAAGCTGGCGCAGGAACAGGCTGAACTGTATATCCCCCTCTAGCTGGCAACTTAGCTCACGCAGGGGCTTCAGTAGACCTGACCATTTTTTCTTTACACTTGGCAGGTGTCTCCTCAATTCTAGGGGCCATTAACTTTATTACAACAATTATCAATATAAAACCCCCTGCCATATCACAATATCAAACCCCTCTATTCGTGTGATCCGTATTAGTCACTGCTGTACTACTACTTCTCTCACTCCCTGTACTAGCAGCCGGAATCACAATACTATTAACAGACCGAAACCTAAATACAACCTTTTTTGACCCAGCAGGAGGCGGAG
An imaged bar code (illuminated Barcode) is shown in fig. 4.
(3) Cervus canadens of Cervus elaphus
DNA sequence (SEQ ID No.7)
TGAGCAGGCATAGTCGGAACAGCCTTAAGCCTACTGATTCGTGCCGAACTGGGCCAACCTGGTACTCTGCTTGGAGACGACCAAATTTATAATGTTATCGTAACCGCACATGCATTCGTAATAATTTTCTTTATAGTTATACCAATTATAATTGGAGGATTTGGTAATTGACTAGTTCCCCTAATAATTGGTGCCCCAGACATAGCATTCCCTCGAATAAACAATATAAGCTTTTGACTCCTCCCTCCTTCTTTCTTACTACTTTTAGCATCATCTATAGTTGAAGCTGGCGCAGGAACAGGCTGAACTGTATACCCCCCTCTAGCTGGCAACTTAGCTCACGCAGGGGCTTCAGTAGACCTAACTATTTTTTCTTTACACTTGGCAGGTGTCTCCTCAATTCTAGGGGCCATTAACTTTATTACAACAATTATTAATATAAAACCCCCTGCCATATCACAATATCAAACCCCTCTATTTGTGTGATCCGTATTAGTCACTGCTGTACTACTACTTCTCTCACTCCCTGTACTAGCAGCCGGAATTACAATACTATTAACAGACCGAAACTTAAATACAACCTTTTTTGACCCAGCAGGAGGCGGAG
An imaged bar code (illuminated Barcode) is shown in fig. 5.
(4) Fallow deer Dama Dama
DNA sequence (SEQ ID No.8)
TGAGCAGGCATAGTCGGAACAGCCTTAAGCCTATTGATTCGTGCTGAACTGGGCCAACCTGGTACCCTACTTGGAGATGACCAAATTTATAATGTTATTGTAACCGCACATGCATTCGTAATAATTTTCTTTATAGTTATACCAATTATAATCGGAGGATTTGGTAACTGACTAGTTCCCTTAATAATTGGTGCCCCAGATATAGCATTCCCTCGAATAAACAATATGAGCTTTTGACTCCTTCCTCCCTCTTTCTTACTACTTCTAGCATCATCTATAGTTGAAGCTGGCGCAGGAACAGGCTGAACTGTGTACCCCCCTCTAGCTGGTAACTTAGCTCACGCAGGAGCCTCAGTGGACCTAACTATCTTTTCTCTACACCTGGCAGGTGTCTCTTCAATTCTAGGGGCCATTAACTTTATTACAACAATTATCAATATAAAACCCCCTGCTATGTCACAATACCAAACTCCCCTATTTGTGTGATCCGTACTAGTCACTGCTGTATTACTACTTCTCTCACTCCCAGTACTAGCAGCTGGAATTACAATATTATTAACAGACCGAAATTTAAATACAACCTTTTTTGATCCAGCAGGAGGCGGAG
An imaged bar code (illuminated Barcode) is shown in fig. 6.
The reference sequence can be used for assisting species identification of related materials (such as antler, traditional Chinese medicine decoction pieces, fossil materials and the like) of the deer animals.
Examples 3-6 species identification Using the specific primer pairs of the invention and reference sequences
Examination of samples of different materials (deer antler, blood or tissue) from four species of cervidae, elk, sika deer, fallow deer and red deer was performed using the specific primer pairs (SEQ ID No.1 and SEQ ID No.2) described in example 1. The method for extracting genome DNA, the PCR amplification system and the method for purifying and sequencing the target fragment in the detection process are shown in example 1. The reference sequence used was the one obtained as described in example 2 above:
(1) elaphurus davidianus
DNA sequence (SEQ ID No.5)
An imaged Barcode (illuminated Barcode) is shown in fig. 3.
(2) Cervus nippon
DNA sequence (SEQ ID No.6)
An imaged bar code (illuminated Barcode) is shown in fig. 4.
(3) Cervus canadens of Cervus elaphus
DNA sequence (SEQ ID No.7)
An imaged bar code (illuminated Barcode) is shown in fig. 5.
(4) Fallow deer Dama Dama
DNA sequence (SEQ ID No.8)
An imaged bar code (illuminated Barcode) is shown in fig. 6.
The result shows that the specific primer has good amplification efficiency in different experimental materials, and the obtained sequence and the imaged bar code can be used for species identification of the cervidae animals and have good identification efficiency.
Sequence listing
Ecological experimental center of <110> Beijing elk
<120> rapid Cervidae animal identification kit based on DNA barcode and application thereof
<130>GAI17CN2264
<160>8
<170>PatentIn version 3.5
<210>1
<211>35
<212>DNA
<213> Artificial sequence
<220>
<223> primer
<400>1
tatttggtgc ctgagcaggc atagtcggaa cagcc 35
<210>2
<211>31
<212>DNA
<213> Artificial sequence
<220>
<223> primer
<400>2
ggtgaccaaa gaatcagaac aagtgttgat a 31
<210>3
<211>25
<212>DNA
<213> Artificial sequence
<220>
<223> primer
<400>3
ggtcaacaaa tcataaagat attgg 25
<210>4
<211>27
<212>DNA
<213> Artificial sequence
<220>
<223> primer
<400>4
taaactttca gggtgaccaa aaaatca 27
<210>5
<211>607
<212>DNA
<213> elk (Elaphurus davidianus)
<400>5
tgagcaggca tagtcggaac agccttaagc ctactgattc gtgctgaatt aggtcaaccc 60
ggtactctgc ttggagatga ccaaatttat aatgttatcg taaccgcaca cgcattcgta 120
ataattttct ttatagttat accaattata attggaggat ttggtaattg actagttccc 180
ctaataattg gtgccccaga tatagcattc cctcgaataa acaatataag cttttgactc 240
ctccctccct ctttcttact acttttagca tcatctatag ttgaagctgg cgcagggaca 300
ggctgaactg tgtatccccc tctagctggc aacctagctc acgcaggagc ttcagtagac 360
ttgactattt tttctttaca tctggcaggt gtctcttcaa ttctgggggc cattaacttt 420
attacaacaa ttattaatat aaaaccccct gctatatcac aatatcaaac ccctctattt 480
gtgtgatccg tactagtcac tgctgtactc ctacttctct cactccctgt actagcagcc 540
ggaattacaa tactattaac agaccgaaac ttaaatacga ccttttttga cccagcagga 600
ggcggag 607
<210>6
<211>607
<212>DNA
<213> Spotted deer (Cervus nippon)
<400>6
tgagcaggca tagtcggaac agccttaagc ctactgattc gtgccgaact gggccaacct 60
ggtactctgc ttggagatga tcaaatttat aatgttatcg taaccgcaca tgcattcgta 120
ataattttct ttatagttat accaattata atcggaggat ttggtaattg actagttccc 180
ctaataattg gtgccccaga catagcattc cctcgaataa acaatataag cttttgactc 240
ctccctcctt ctttcttact acttttagca tcatctatag ttgaagctgg cgcaggaaca 300
ggctgaactg tatatccccc tctagctggc aacttagctc acgcaggggc ttcagtagac 360
ctgaccattt tttctttaca cttggcaggt gtctcctcaa ttctaggggc cattaacttt 420
attacaacaa ttatcaatat aaaaccccct gccatatcac aatatcaaac ccctctattc 480
gtgtgatccg tattagtcac tgctgtacta ctacttctct cactccctgt actagcagcc 540
ggaatcacaa tactattaac agaccgaaac ctaaatacaa ccttttttga cccagcagga 600
ggcggag 607
<210>7
<211>607
<212>DNA
<213> red deer (Cervus canadens)
<400>7
tgagcaggca tagtcggaac agccttaagc ctactgattc gtgccgaact gggccaacct 60
ggtactctgc ttggagacga ccaaatttat aatgttatcg taaccgcaca tgcattcgta 120
ataattttct ttatagttat accaattata attggaggat ttggtaattg actagttccc 180
ctaataattg gtgccccaga catagcattc cctcgaataa acaatataag cttttgactc 240
ctccctcctt ctttcttact acttttagca tcatctatag ttgaagctgg cgcaggaaca 300
ggctgaactg tatacccccc tctagctggc aacttagctc acgcaggggc ttcagtagac 360
ctaactattt tttctttaca cttggcaggt gtctcctcaa ttctaggggc cattaacttt 420
attacaacaa ttattaatat aaaaccccct gccatatcac aatatcaaac ccctctattt 480
gtgtgatccg tattagtcac tgctgtacta ctacttctct cactccctgt actagcagcc 540
ggaattacaa tactattaac agaccgaaac ttaaatacaa ccttttttga cccagcagga 600
ggcggag 607
<210>8
<211>607
<212>DNA
<213> fallow deer (Dama Dama)
<400>8
tgagcaggca tagtcggaac agccttaagc ctattgattc gtgctgaact gggccaacct 60
ggtaccctac ttggagatga ccaaatttat aatgttattg taaccgcaca tgcattcgta 120
ataattttct ttatagttat accaattata atcggaggat ttggtaactg actagttccc 180
ttaataattg gtgccccaga tatagcattc cctcgaataa acaatatgag cttttgactc 240
cttcctccct ctttcttact acttctagca tcatctatag ttgaagctgg cgcaggaaca 300
ggctgaactg tgtacccccc tctagctggt aacttagctc acgcaggagc ctcagtggac 360
ctaactatct tttctctaca cctggcaggt gtctcttcaa ttctaggggc cattaacttt 420
attacaacaa ttatcaatat aaaaccccct gctatgtcac aataccaaac tcccctattt 480
gtgtgatccg tactagtcac tgctgtatta ctacttctct cactcccagt actagcagct 540
ggaattacaa tattattaac agaccgaaat ttaaatacaa ccttttttga tccagcagga 600
ggcggag 607

Claims (11)

1. A cervidae animal identification kit comprising the following four labeled or unlabeled DNA sequences or barcodes thereof:
SEQ ID No.5、SEQ ID No.6、SEQ ID No.7、SEQ ID No.8。
2. the kit according to claim 1, which comprises the barcode shown in fig. 3, fig. 4, fig. 5 and fig. 6, wherein the DNA sequence of the barcode shown in fig. 3 is shown as SEQ ID No.5, the DNA sequence of the barcode shown in fig. 4 is shown as SEQ ID No.6, the DNA sequence of the barcode shown in fig. 5 is shown as SEQ ID No.7, and the DNA sequence of the barcode shown in fig. 6 is shown as SEQ ID No. 8.
3. The kit of claim 1, further comprising the following primers:
SEQ ID No.1(5’-3’):TATTTGGTGCCTGAGCAGGCATAGTCGGAACAGCC;
SEQ ID No.2(5’-3’):GGTGACCAAAGAATCAGAACAAGTGTTGATA。
4. the kit of claim 2, further comprising a molecular systems tree.
5. Use of the kit of any one of claims 1 to 4 for identifying a species of cervidae animals.
6. Use according to claim 5, wherein said kit comprises an imaged barcode of the sequence shown in SEQ ID No.5, for identifying the presence or absence of elk components in a sample to be tested.
7. The use of claim 5, wherein the kit comprises an imaged barcode of the sequence shown in SEQ ID No.6, and is used for identifying the presence of Cervus Nippon Temminck components in a sample to be tested.
8. Use according to claim 5, wherein the kit comprises an imaged barcode of the sequence shown in SEQ ID No.7, for identifying the presence of Cervus elaphus components in a sample to be tested.
9. Use according to claim 5, wherein the kit comprises an imaged barcode of the sequence shown in SEQ ID No.8 for identifying the presence of fallow deer components in a sample to be tested.
10. The use according to any one of claims 6 to 9, wherein the sample to be tested is a medicinal material, a Chinese medicinal preparation or a fossil material which is required to identify whether or not the sample contains a component of a cervidae animal and/or is required to identify a species of the cervidae animal.
11. The use according to claim 10, wherein the sample to be tested is deer horn, blood or tissue, or a herbal piece of raw materials for identification of deer components and/or species.
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