CN1363660A - Polypeptide-human glutamyl transfer RNA synthetase 23.76 and polynucleotide for coding it - Google Patents
Polypeptide-human glutamyl transfer RNA synthetase 23.76 and polynucleotide for coding it Download PDFInfo
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Abstract
A novel polypeptide-human glutamyl tRNA synthetase 23.76, the polynucleotide for coding it, the process for preparing said polypeptide by DNA recombination, the application of said polypeptide in treating diseases such as cancer, HIV infection, etc, the antagon of said polypeptide and its medical function, and the application of said polynucleotide are disclosed.
Description
The invention belongs to biological technical field, specifically, the invention describes a kind of new polypeptide-human glutamy tRNA synthetic enzyme 23.76, and the polynucleotide sequence of this polypeptide of encoding.The invention still further relates to the preparation method and the application of these polynucleotide and polypeptide.
The protein information of DNA institute load generates the part that mRNA has only finished genetic expression by Transcription, and a more complicated part is exactly a translation process, and nucleic acid language shift just is the process of protein language.Dominant role in this process has various aminoacyl-tRNA synthetases, various tRNA and rrna.Because their acting in conjunction, amino acid could interconnect according to the information that mRNA provided becomes polypeptide chain.
It is amino acid, tRNA, ATP that aminoacyl-tRNA synthetase (aaRS) has three substrates.The esterification of aaRS catalytic amino acid makes it to be connected in the 3 ' end of tRNA, and each aaRS is corresponding to a seed amino acid and several isoaccepting tRNAs.ATP provides activated amino acid required energy, and amino acid activation earlier is aminoacyl adenylate, and then generates aminoacyl-tRNA with tRNA.Interact between aaRS and the substrate and relate to identification and bonded problem.
AaRS can be divided into two types that respectively contain ten members, and glutamy tRNA synthetic enzyme belongs to aaRS Class1 (Eriani et al., 1990).The aaRS Class1 has following structural domain (Cavarelli J etal., 1998) usually:
1. amino acid identified region: at aaRS Class1 amino acid the amino-acid residue of two high conservatives is only arranged in conjunction with the crack, one be tyrosine residues in 347 sites, one is that asparagicacid residue is in 191 sites.At ArgRS, Tyr347 participates in the η-nitrogen-atoms of identification amino acid substrate, and in other member of aaRS Class1, tyrosine residues is carried out some other function.Asp191 is at the C of the 5th βZhe Die of chain end, and it does not relate to substrate in conjunction with but structural effect being arranged, and it has stablized the 5th βZhe Die of chain and the 6th βZhe Die of chain and the interaction of secondary structure on every side.
2.ATP binding site: two special polypeptide structure territory HIGH and KMSKS are connected in ATP-binding site.The last constant Gly of HIGH has formed a platform so that in conjunction with ATP at the N of the 6th α spiral of chain end, and two His and Lys relate to stablizing that aminoacylation transition state product forms.
3.tRNA identification and binding site: Add-1 and Add-2 structural domain corecognition anticodon and tRNA arm, structural domain Ins-1 has hidden one side of amino acid receptor trunk, the folding the other side that hidden of Rossmann.
4.tRNA grappling platform: the member of aaRS Class1 is by the 13rd βZhe Die of a chain and the 14th structural domain that βZhe Die is formed of chain, be positioned at Rossmann folding after, this structural domain relates to tRNA and is anchored to glutamy tRNA synthetic enzyme platform.
5.ArgRS the RNA of N end is in conjunction with the territory: the Add-1 structural domain of glutamy tRNA synthetic enzyme and the identification of tRNA, the closest with the interaction of the D puff Lu of tRNA.The exposed βZhe Die of Add-1 structural domain occupies vital role on many nucleic acid binding proteins.
6. anticodon binding site: the anticodon binding site of glutamy tRNA synthetic enzyme is positioned at the left-hand side of C end, and the exposed βZhe Die of Add-1 structural domain is also discerned anticodon arm.
Studies show that nine aaRS (Arg, Asp, Gln, Glu, Ile, Leu, Lys, Met, and Pro) are by a genes encoding (Vellekamp et al., 1985).
Glutamy tRNA synthetic enzyme catalysis L-glutamic acid isoaccepting tRNA carries L-glutamic acid, in the presence of the rrna and the relevant factor, finish peptide chain initial, extend and stop.
The polynucleotide of coding human glutaminyl tRNA synthetic enzyme, and coded human glutaminyl tRNA synthetic enzyme be found to be the differentiation of research cell under normal and pathological conditions, the physiological and biochemical procedure of propagation provides a kind of method, also comprises that with the disease that the disorder of cytodifferentiation propagation causes cancer provides a kind of new way for diagnosis, treatment.
According to amino acid homology result relatively, polypeptide of the present invention is accredited as human glutaminyl tRNA synthetic enzyme 23.76 (HGluRS58) or human glutaminyl tRNA transaminase 58 (HGluAT58) by deduction, its human glutaminyl tRNA synthetic enzyme is the glutamy tRNA transaminase of a kind of rickettsia, and albumen number is AJ235270.
Analysis by gene chip is found, at normal brain activity, liver cancer, muscle, tire brain, tire kidney, in tire lung, tire liver, Tiroidina, thymus gland, adult liver, lung, the glioma, polypeptide expression spectrum of the present invention is very approximate with the express spectra of human glutaminyl tRNA synthetic enzyme, so the two function also may be similar.The present invention is named as human glutaminyl tRNA synthetic enzyme 23.76.
Because human glutaminyl tRNA synthetic enzyme 23.76 albumen play an important role in regulating body critical functions such as cell fission and fetal development as mentioned above, and believe and relate to a large amount of albumen in these regulate processes, thereby need to identify human glutaminyl tRNA synthetic enzyme 23.76 albumen of more these processes of participation in this area always, particularly identify this proteic aminoacid sequence.The separation of new human glutaminyl tRNA synthetic enzyme 23.76 protein coding genes also provides the foundation for determining the effect of this albumen under healthy and morbid state.This albumen may constitute the basis of 1 sick diagnosis of exploitation disease and/or curative, and it is very important therefore separating its coding DNA.
An object of the present invention is to provide isolating new polypeptide-human glutamy tRNA synthetic enzyme 23.76 with and fragment, analogue and derivative.
Another object of the present invention provides the polynucleotide of this polypeptide of coding.
Another object of the present invention provides the recombinant vectors of the polynucleotide that contain coding human glutaminyl tRNA synthetic enzyme 23.76.
Another object of the present invention provides the genetically engineered host cell of the polynucleotide that contain coding human glutaminyl tRNA synthetic enzyme 23.76.
Another object of the present invention provides the method for producing human glutaminyl tRNA synthetic enzyme 23.76.
Another object of the present invention provides the antibody at polypeptide-human glutamy tRNA synthetic enzyme 23.76 of the present invention.
Another object of the present invention has provided simulated compound, antagonist, agonist, the inhibitor at polypeptide-human glutamy tRNA synthetic enzyme 23.76 of the present invention.
Another object of the present invention provides the method for the unusual relevant disease of diagnoses and treatment and human glutaminyl tRNA synthetic enzyme 23.76.
The present invention relates to a kind of isolated polypeptide, this polypeptide is the people source, and it comprises: polypeptide or its examples of conservative variations, bioactive fragment or derivative with SEQ ID No.2 aminoacid sequence.Preferably, this polypeptide is the polypeptide with SEQ ID NO:2 aminoacid sequence.
The invention still further relates to a kind of isolating polynucleotide, it comprises a kind of nucleotide sequence or its variant that is selected from down group:
(a) coding has the polynucleotide of the polypeptide of SEQ ID No.2 aminoacid sequence;
(b) with polynucleotide (a) complementary polynucleotide;
(c) with (a) or polynucleotide sequence (b) have the polynucleotide of at least 70% homogeny.
More preferably, the sequence of these polynucleotide is be selected from down group a kind of: the sequence that (a) has 83-733 position among the SEQ ID NO:1; (b) has the sequence of 1-4070 position among the SEQ ID NO:1.
The present invention relates to a kind of carrier that contains polynucleotide of the present invention, particularly expression vector in addition; The host cell that this carrier of a kind of usefulness is genetically engineered comprises the host cell of conversion, transduction or transfection; A kind of method for preparing polypeptide of the present invention of cultivating described host cell and reclaiming expression product that comprises.
The invention still further relates to a kind of can with polypeptid specificity bonded antibody of the present invention.
The invention still further relates to a kind of simulation, activation, antagonism of screening or suppress the method for the compound of human glutaminyl tRNA synthetic enzyme 23.76 protein-actives, it comprises and utilizes polypeptide of the present invention.The invention still further relates to the compound that obtains with this method.
The invention still further relates to a kind of vitro detection and express the relevant disease or the method for disease susceptibility with human glutaminyl tRNA synthetic enzyme 23.76 abnormal proteins, comprise the sudden change in polypeptide described in the detection of biological sample or its coded polynucleotide sequence, perhaps the amount or the biological activity of polypeptide of the present invention in the detection of biological sample.
The present invention also relates to a kind of pharmaceutical composition, it contains polypeptide of the present invention or its stand-in, activator, antagonist or inhibitor and pharmaceutically acceptable carrier.
The invention still further relates to polypeptide of the present invention and/or polynucleotide and be used for the treatment of cancer, developmental character disease or immunological disease or other purposes owing to the medicine of human glutaminyl tRNA synthetic enzyme 23.76 diseases that abnormal expression causes in preparation.
Others of the present invention are because disclosing of the technology of this paper is conspicuous to those skilled in the art.
The following term of using in this specification sheets and claims has following implication unless stated otherwise:
" nucleotide sequence " is meant oligonucleotide, Nucleotide or polynucleotide and fragment or part, also can refer to genome or synthetic DNA or RNA, and they can be strand or two strands, represent sense strand or antisense strand.Similarly, term " aminoacid sequence " is meant oligopeptides, peptide, polypeptide or protein sequence and fragment or part.When " aminoacid sequence " among the present invention related to a kind of aminoacid sequence of naturally occurring protein molecule, this " polypeptide " or " protein " did not mean that aminoacid sequence are restricted to the complete natural amino acid relevant with described protein molecule.
Protein or polynucleotide " variant " are meant a kind of polynucleotide sequence that has the aminoacid sequence of one or more amino acid or Nucleotide change or encode it.Described change can comprise disappearance, insertion or the replacement of amino acid in aminoacid sequence or the nucleotide sequence or Nucleotide.Variant can have " conservative property " and change, and wherein the amino acid of Ti Huaning has structure or the chemical property similar with original acid, as replacing Isoleucine with leucine.Variant also can have non-conservation and change, as replacing glycine with tryptophane.
" disappearance " is meant the disappearance of in aminoacid sequence or nucleotide sequence one or more amino acid or Nucleotide.
" insertion " or " interpolation " is meant that the change in aminoacid sequence or nucleotide sequence causes comparing the increase of one or more amino acid or Nucleotide with naturally occurring molecule." replacement " is meant by different amino acid or Nucleotide and replaces one or more amino acid or Nucleotide.
" biological activity " is meant the protein of structure, regulation and control or biochemical function with natural molecule.Similarly, term " immunologic competence " be meant natural, reorganization or synthetic protein and fragment thereof in suitable animal or cell, induce specific immune response and with specific antibody bonded ability.
" agonist " is meant when combining with human glutaminyl tRNA synthetic enzyme 23.76, thereby a kind of this protein that causes changes the molecule of regulating this protein active.Agonist can comprise protein, nucleic acid, carbohydrate or any other can be in conjunction with the molecule of human glutaminyl tRNA synthetic enzyme 23.76.
" antagonist " or " inhibition " is meant when combining with human glutaminyl tRNA synthetic enzyme 23.76, a kind of sealing or the biologic activity of mediator's glutamy tRNA synthetic enzyme 23.76 or the molecule of immunologic competence.Antagonist and inhibition can comprise protein, nucleic acid, carbohydrate or any other can be in conjunction with the molecule of human glutaminyl tRNA synthetic enzyme 23.76.
" adjusting " is meant that the function of human glutaminyl tRNA synthetic enzyme 23.76 changes, and comprises the change of any other biological property, function or the immune property of the change of the rising of protein active or reduction, binding characteristic and human glutaminyl tRNA synthetic enzyme 23.76.
The pure basically " of " is meant and is substantially free of natural relative other albumen, lipid, carbohydrate or other material.Those skilled in the art can use the purified technology of protein purifying human glutaminyl tRNA synthetic enzyme 23.76 of standard.Basically pure human glutaminyl tRNA synthetic enzyme 23.76 can produce single master tape on the irreducibility polyacrylamide gel.The purity available amino end acid sequence of human glutaminyl tRNA synthetic enzyme 23.76 polypeptide is analyzed.
" complementary " or " complementation " is meant under salt concn that allows and temperature condition by the natural combination of the polynucleotide of base pairing.For example, sequence " C-T-G-A " can combine with complementary sequence " G-A-C-T ".Complementation between two single chain molecules can be part or whole.Complementary degree between the nucleic acid chains has a significant effect for efficient of hybridizing between the nucleic acid chains and intensity.
" homology " is meant the complementary degree, can be portion homologous or complete homology." portion homologous " is meant a kind of part complementary sequence, and it can partly suppress the hybridization of complete complementary sequence and target nucleic acid at least.The inhibition of this hybridization can detect by hybridizing (Southern trace or Northern trace etc.) under the condition that reduces in the severity degree.Basically homologous sequence or hybridization probe can compete and suppress complete homologous sequence and target sequence the condition that reduces of severity degree under combine.This does not mean the conditions permit non-specific binding that the severity degree reduces because the conditional request two sequences that the severity degree reduces mutual be combined into specificity or selectivity interacts.
" homogeny percentage " be meant two or more amino acid or nucleotide sequence relatively in the same or analogous percentage of sequence.The available electron method is measured the homogeny percentage, as passing through MEGALIGN program (Lasergenesoftware package, DNASTAR, Inc., Madison Wis.).The MEGALIGN program can compare two or more sequences (Higgins, D.G. and P.M.Sharp (1988) Gene 73:237-244) according to diverse ways such as Cluster method.The Cluster method is organized the series arrangement cluster by checking the distance between all pairings with each.Then with each bunch with in pairs or become set of dispense.Homogeny percentage between two aminoacid sequences such as sequence A and the sequence B calculates by following formula:
Also can be by the Cluster method or with the homogeny percentage (Hein J., (1990) Methods in emzumology 183:625-645) between known method in this area such as the Jotun Hein mensuration nucleotide sequence.
" similarity " is meant the degree that the identical or conservative property of corresponding position amino-acid residue when arranging contrast between the aminoacid sequence replaces.For example be used for amino acid that conservative property replaces, electronegative amino acid can comprise aspartic acid and L-glutamic acid; Positively charged amino acid can comprise Methionin and arginine; Having uncharged head group has similar hydrophilic amino acid can comprise leucine, Isoleucine and Xie Ansuan; Glycine and L-Ala; L-asparagine and glutamine; Serine and Threonine; Phenylalanine and tyrosine.
" antisense " is meant and specific DNA or RNA sequence complementary nucleotide sequence." antisense strand " is meant and " sense strand " complementary nucleic acid chains.
" derivative " is meant HFP or encodes its chemical modification object of nucleic acid.This chemical modification object can be with alkyl, acyl group or the amino hydrogen atom of replacing.The nucleic acid derivative codified keeps the polypeptide of the main biological characteristics of natural molecule.
" antibody " is meant complete antibody molecule and fragment thereof, as Fa, F (ab ')
2And Fv, its energy specificity is in conjunction with the antigenic determinant of human glutaminyl tRNA synthetic enzyme 23.76.
" humanized antibody " is meant that the aminoacid sequence in non-antigen binding domain territory is replaced and becomes more similar to people's antibody, but still keep original in active antibody.
" isolating " speech refers to material is shifted out among its original environment (for example, if spontaneous its natural surroundings that just refers to).Such as it is exactly not to be separated that spontaneous polynucleotide or polypeptide are present in the Live Animals, but same polynucleotide or polypeptide with some or all in natural system with it the material of coexistence separately be exactly isolating.Such polynucleotide may be the parts of a certain carrier, the part that also possible such polynucleotide or polypeptide are a certain composition.Since carrier or composition are not the compositions of its natural surroundings, they remain isolating.
As used herein, " isolating " are meant that material separates (if natural substance, primal environment promptly is a natural surroundings) from its primal environment.Do not have separation and purification as polynucleotide under the native state in the active somatic cell and polypeptide, but same polynucleotide or polypeptide as from native state with in other materials that exist separately, then for separation and purification.
As used herein, " isolating human glutaminyl tRNA synthetic enzyme 23.76 " is meant that human glutaminyl tRNA synthetic enzyme 23.76 is substantially free of natural relative other albumen, lipid, carbohydrate or other material.Those skilled in the art can use the purified technology of protein purifying human glutaminyl tRNA synthetic enzyme 23.76 of standard.Basically pure polypeptide can produce single master tape on non-reduced polyacrylamide gel.The purity of human glutaminyl tRNA synthetic enzyme 23.76 polypeptide can be used amino acid sequence analysis.
The invention provides a kind of new polypeptide-human glutamy tRNA synthetic enzyme 23.76, it is made up of the aminoacid sequence shown in the SEQID NO:2 basically.Polypeptide of the present invention can be recombinant polypeptide, natural polypeptides, synthetic polypeptide, preferred recombinant polypeptide.Polypeptide of the present invention can be the product of natural purifying, or the product of chemosynthesis, or uses recombinant technology to produce from protokaryon or eucaryon host (for example, bacterium, yeast, higher plant, insect and mammalian cell).The host used according to the recombinant production scheme, polypeptide of the present invention can be glycosylated, maybe can be nonglycosylated.Polypeptide of the present invention also can comprise or not comprise initial methionine residues.
The present invention also comprises fragment, derivative and the analogue of human glutaminyl tRNA synthetic enzyme 23.76.As used herein, term " fragment ", " derivative " and " analogue " are meant biological function or the active polypeptide that keeps human glutaminyl tRNA synthetic enzyme of the present invention 23.76 identical basically.The fragment of polypeptide of the present invention, derivative or analogue can be: (I) a kind of like this, wherein one or more amino-acid residues are replaced by conservative or non-conservative amino acid residues (preferably conservative amino acid residues), and the amino acid that replaces can be also can not encoded by genetic codon; Perhaps (II) is a kind of like this, and certain group on wherein one or more amino-acid residues is replaced by other group and comprises substituting group; Perhaps (III) is a kind of like this, and wherein mature polypeptide and another kind of compound (such as the compound that prolongs the polypeptide transformation period, for example polyoxyethylene glycol) merge; Perhaps (IV) is a kind of like this, wherein additional aminoacid sequence is integrated into mature polypeptide and the peptide sequence that forms (as leader sequence or secretion sequence or be used for the sequence or the proteinogen sequence of this polypeptide of purifying) by the elaboration of this paper, such fragment, 00 derivative and analogue are considered within those skilled in the art's ken.
The invention provides isolating nucleic acid (polynucleotide), substantially the polynucleotide that have a polypeptide of SEQ ID NO:2 aminoacid sequence by coding are formed.Polynucleotide sequence of the present invention comprises the nucleotide sequence of SEQ ID NO:1.Polynucleotide of the present invention are to find from the cDNA library of people's fetal brain tissue.The polynucleotide sequence total length that it comprises is 4070 bases, its open reading frame 83-733 216 amino acid of having encoded.Find relatively that according to gene chip expression spectral this polypeptide has similar express spectra to human glutaminyl tRNA synthetic enzyme, deducibility goes out this human glutaminyl tRNA synthetic enzyme 23.76 and has the similar function of human glutaminyl tRNA synthetic enzyme.
Polynucleotide of the present invention can be dna form or rna form.Dna form comprises the DNA of cDNA, genomic dna or synthetic.DNA can be strand or double-stranded.DNA can be coding strand or noncoding strand.The coding region sequence of encoding mature polypeptide can be identical with the coding region sequence shown in the SEQ ID NO:1 or the varient of degeneracy.As used herein, " varient of degeneracy " are meant that in the present invention coding has protein or the polypeptide of SEQ ID NO:2, but with the differentiated nucleotide sequence of coding region sequence shown in the SEQ ID NO:1.
The polynucleotide of the mature polypeptide of coding SEQ ID NO:2 comprise: the encoding sequence that has only mature polypeptide; The encoding sequence of mature polypeptide and various additional code sequence; Encoding sequence of mature polypeptide (with optional additional code sequence) and non-coding sequence.
Term " polynucleotide of coded polypeptide " is meant polynucleotide that comprise this polypeptide of encoding and the polynucleotide that comprise additional code and/or non-coding sequence.
The invention still further relates to the varient of foregoing description polynucleotide, its coding has the polypeptide of identical aminoacid sequence or segment, analogue and the derivative of polypeptide with the present invention.The varient of these polynucleotide can be the allelic variant of natural generation or the varient that non-natural takes place.These nucleotide diversity bodies comprise and replace varient, deletion mutation body and insert varient.As known in the art, allelic variant is the replacement form of polynucleotide, and it may be replacement, disappearance or the insertion of one or more Nucleotide, but can be from not changing the function of its encoded polypeptides in fact.
The invention still further relates to and the polynucleotide (have at least 50% between two sequences, preferably have 70% homogeny) of sequence hybridization described above.The present invention be more particularly directed under stringent condition and the interfertile polynucleotide of polynucleotide of the present invention.In the present invention, " stringent condition " is meant: (1) than hybridization under low ionic strength and the comparatively high temps and wash-out, as 0.2 * SSC, and 0.1%SDS, 60 ℃; Or (2) hybridization the time adds and to use denaturing agent, as 50% (v/v) methane amide, 0.1% calf serum/0.1%Ficoll, 42 ℃ etc.; Or (3) only at the homogeny between the two sequences at least more than 95%, be more preferably 97% and just hybridize when above.And the polypeptide of interfertile polynucleotide encoding has identical biological function and activity with the mature polypeptide shown in the SEQ ID NO:2.
The invention still further relates to nucleic acid fragment with sequence hybridization described above.As used herein, the length of " nucleic acid fragment " contain 10 Nucleotide at least, better are 20-30 Nucleotide at least, are more preferably 50-60 Nucleotide at least, preferably more than at least 100 Nucleotide.Nucleic acid fragment also can be used for the amplification technique (as PCR) of nucleic acid to determine and/or to separate the polynucleotide of coding human glutaminyl tRNA synthetic enzyme 23.76.
Polypeptide among the present invention and polynucleotide preferably provide with isolating form, more preferably are purified to homogeneous.
The special polynucleotide sequence of coding human glutaminyl tRNA synthetic enzyme 23.76 of the present invention can obtain with several different methods.For example, separate polynucleotide with hybridization technique well known in the art.These technology including, but not limited to: 1) with probe and genome or the hybridization of cDNA library to detect homologous polynucleotide sequence and 2) antibody screening of expression library to be to detect the polynucleotide passage of the clone with common structure feature.
Sequence dna fragment of the present invention also can obtain with following method: 1) separate double chain DNA sequence from genomic dna; 2) the chemical synthesising DNA sequence is to obtain the double-stranded DNA of described polypeptide.
In the above-mentioned method of mentioning, isolation of genomic DNA is least commonly used.The direct chemical of dna sequence dna is synthetic to be the method for often selecting for use.The more frequent method of selecting for use is the separation of cDNA sequence.The standard method that separates interested cDNA is from the donorcells separating mRNA of this gene of high expression level and carries out reverse transcription, forms plasmid or phage cDNA library.Extract the existing multiple proven technique of method of mRNA, test kit also can obtain (Qiagene) from commercial channels.And the construction cDNA library also is usual method (Sambrook, et al., MolecularCloning, A Laboratory Manual, Cold Spring Harbor Laboratory.New York, 1989).Also can obtain the cDNA library of commercial offers, as the different cDNA library of Clontech company.When being used in combination the polymeric enzyme reaction technology, even few expression product also can be cloned.
Available ordinary method is screened gene of the present invention from these cDNA libraries.These methods include, but is not limited to: (1) DNA-DNA or DNA-RNA hybridization; (2) appearance of marker gene function or forfeiture; (3) level of the transcript of mensuration human glutaminyl tRNA synthetic enzyme 23.76; (4), detect the protein product of genetic expression by immunological technique or mensuration biologic activity.Aforesaid method can singly be used, but also several different methods combined utilization.
In (1) kind method, hybridizing used probe is and any a part of homology of polynucleotide of the present invention that at least 10 Nucleotide of its length better are at least 30 Nucleotide, are more preferably at least 50 Nucleotide, preferably at least 100 Nucleotide.In addition, within 2000 Nucleotide, preferable is within 1000 Nucleotide to the length of probe usually.Probe used herein is the dna sequence dna of chemosynthesis on the basis of gene order information of the present invention normally.Gene of the present invention itself or fragment are certainly as probe.The mark of dna probe can be used radio isotope, fluorescein or enzyme (as alkaline phosphatase) etc.
In (4) kind method, detect the protein product of human glutaminyl tRNA synthetic enzyme 23.76 genetic expressions and can use immunological technique such as Western blotting, radioimmunoprecipitation, enzyme-linked immunosorbent assay (ELISA) etc.
Use method (Saiki, the et al.Science1985 of round pcr DNA amplification/RNA; 230:1350-1354) be optimized for acquisition gene of the present invention.When particularly being difficult to from the library, obtain the cDNA of total length, can preferably use RACE method (the terminal rapid amplifying method of RACE-cDNA), the primer that is used for PCR can suitably be selected according to polynucleotide sequence information of the present invention disclosed herein, and available ordinary method is synthetic.Available ordinary method is as the DNA/RNA fragment by gel electrophoresis separation and purifying amplification.
The gene of the present invention that obtains as mentioned above, perhaps the polynucleotide sequence of various dna fragmentations etc. can with ordinary method such as dideoxy chain termination (Sanger et al.PNAS, 1977,74:5463-5467) measure.This class polynucleotide sequence is measured also available commercial sequencing kit etc.In order to obtain the cDNA sequence of total length, order-checking need be carried out repeatedly.Sometimes need to measure a plurality of clones' cDNA sequence, just can be spliced into the cDNA sequence of total length.
The present invention also relates to comprise the carrier of polynucleotide of the present invention, and with carrier of the present invention or directly with the host cell of human glutaminyl tRNA synthetic enzyme 23.76 encoding sequences, and the method that produces polypeptide of the present invention through recombinant technology through the genetically engineered generation.
Among the present invention, the polynucleotide sequence of coding human glutaminyl tRNA synthetic enzyme 23.76 can be inserted in the carrier, contains the recombinant vectors of polynucleotide of the present invention with formation.Term " carrier " refers to that bacterial plasmid well known in the art, phage, yeast plasmid, vegetable cell virus, mammalian cell virus are as adenovirus, retrovirus or other carrier.The carrier of Shi Yonging includes but not limited in the present invention: and the expression vector based on the T7 promotor of in bacterium, expressing (Rosenberg, et al.Gene, 1987,56:125); The pMSXND expression vector of in mammalian cell, expressing (Lee and Nathans, J Bio Chem.263:3521,1988) and at the carrier that derives from baculovirus of expressed in insect cells.In a word, as long as can duplicate in host and stablize, any plasmid and carrier may be used to make up recombinant expression vector.A key character of expression vector is to contain replication origin, promotor, marker gene and translational control element usually.
Method well-known to those having ordinary skill in the art can be used to make up the dna sequence dna that contains coding human glutaminyl tRNA synthetic enzyme 23.76 and the expression vector of suitable transcribing/translational control element.These methods comprise (Sambroook, et al.Molecular Cloning, aLaboratory Manual, cold Spring Harbor Laboratory.New York, 1989) such as extracorporeal recombinant DNA technology, DNA synthetic technology, the interior recombinant technologys of body.Described dna sequence dna can effectively be connected on the suitable promotor in the expression vector, and is synthetic to instruct mRNA.The representative example of these promotors has: colibacillary lac or trp promotor; The P of lambda particles phage
LPromotor; Eukaryotic promoter comprises LTRs and some other known may command gene expression promoter in prokaryotic cell prokaryocyte or eukaryotic cell or its virus of CMV immediate early promoter, HSV thymidine kinase promoter, early stage and late period SV40 promotor, retrovirus.Expression vector also comprises ribosome bind site that translation initiation is used and transcription terminator etc.Inserting enhancer sequence in carrier will make its transcribing in higher eucaryotic cells be enhanced.Enhanser is the cis acting factor that DNA expresses, and nearly 10 to 300 base pairs act on promotor transcribing with enhancing gene usually.Can for example be included in the SV40 enhanser of 100 to 270 base pairs of replication origin side in late period one, at the polyoma enhanser of replication origin side in late period one and adenovirus enhanser etc.
In addition, expression vector preferably comprises one or more selected markers, to be provided for selecting the phenotypic character of transformed host cells, cultivate Tetrahydrofolate dehydrogenase, neomycin resistance and the green fluorescent protein (GFP) of usefulness as eukaryotic cell, or be used for colibacillary tsiklomitsin or amicillin resistance etc.
Persons skilled in the art all know how to select appropriate carriers/transcriptional regulatory element (as promotor, enhanser etc.) and selected marker.
Among the present invention, the polynucleotide of coding human glutaminyl tRNA synthetic enzyme 23.76 or the recombinant vectors that contains these polynucleotide can transform or transduce into host cell, contain the genetically engineered host cell of these polynucleotide or recombinant vectors with formation.Term " host cell " refers to prokaryotic cell prokaryocyte, as bacterial cell; Or eukaryotic cell such as low, as yeast cell; Or higher eucaryotic cells, as mammalian cell.Representative example has: intestinal bacteria, streptomyces; Bacterial cell such as Salmonella typhimurium; Fungal cell such as yeast; Vegetable cell; Insect cell such as fruit bat S2 or Sf9; Zooblast such as CHO, COS or Bowes melanoma cells etc.
Can carry out with routine techniques well known to those skilled in the art with dna sequence dna of the present invention or the recombinant vectors transformed host cell that contains described dna sequence dna.When the host was prokaryotic organism such as intestinal bacteria, the competent cell that can absorb DNA can be used CaCl in exponential growth after date results
2Method is handled, and used step is well-known in this area.Alternative is to use MgCl
2If desired, transforming also the method for available electroporation carries out.When the host is an eukaryote, can select following DNA transfection method for use: coprecipitation of calcium phosphate method, perhaps conventional mechanical method such as microinjection, electroporation, liposome packing etc.
By the recombinant DNA technology of routine, utilize polynucleotide sequence of the present invention to can be used to express or produce human glutaminyl tRNA synthetic enzyme 23.76 (Science, 1984 of reorganization; 224:1431).In general following steps are arranged:
(1). with the polynucleotide (or varient) of coding of the present invention people human glutaminyl tRNA synthetic enzyme 23.76, or with the recombinant expression vector that contains these polynucleotide proper host cell that transforms or transduce;
(2). in suitable medium, cultivate host cell;
(3). separation, protein purification from substratum or cell.
In step (2), according to used host cell, used substratum can be selected from various conventional substratum in the cultivation.Under the condition that is suitable for the host cell growth, cultivate.After host cell grows into suitable cell density, induce the promotor of selection with suitable method (as temperature transition or chemical induction), cell is cultivated for some time again.
In step (3), recombinant polypeptide can wrap and be expressed or be secreted into the extracellular in cell or on cytolemma.If desired, can utilize its physics, the separating by various separation methods with other characteristic and the albumen of purification of Recombinant of chemistry.These methods are well-known to those skilled in the art.These methods include, but are not limited to: conventional renaturation is handled, protein precipitant is handled (salt analysis method), centrifugal, the broken bacterium of infiltration, the combination of ultrasonication, super centrifugal, sieve chromatography (gel-filtration), adsorption chromatography, ion exchange chromatography, high performance liquid chromatography (HPLC) and other various liquid chromatography (LC) technology and these methods.
The antagonist of polypeptide of the present invention and this polypeptide, agonist and inhibitor can be directly used in disease treatment, for example, can treat malignant tumour, adrenal gland defect, tetter, all kinds of inflammation, HIV infection and immunological disease etc.
Polypeptide of the present invention (human glutaminyl tRNA synthetic enzyme 23.76) is absolutely necessary in proteinic building-up process, and its existence has and important meaning for proteinic translation.The abnormal expression of human glutaminyl tRNA synthetic enzyme 23.76 of the present invention will produce proteinic biosynthesizing obstacle, and produce various diseases thus.These diseases include but not limited to:
Grow disorders, as spina bifida, the cranium fissure, anencephalia, the brain bulging, the hole deformity of brain, congenital hydrocephalus, the aqueduct deformity, achondroplastic dwarf's disease, spondyloepiphyseal dysplasia disease, the Langer-Giedion syndromes, hypogenitalism, epispadia, latent, with malformation syndrome of short and small stature such as Conradi syndromes and Danbolt-Closs syndromes, congenital glaucoma or cataract, congenital little fissura palpebrae, retinal development is unusual, atrophia nervi optici congenita, ulcuscuris, monster, the Williams syndromes, the Alagille syndromes, shellfish syndrome Weis two;
Metabolism and nutritive disease, as atrophy, hyperlipidaemia and hyperlipoproteinemia, obesity, deficiency disease;
Inflammation is as atopic reaction, adult respiratory distress syndrome, lung eosinophilia, rheumatoid arthritis, similar rheumatism sample sacroiliitis, cholecystitis, glomerulonephritis, dermatomyositis, polymyositis, Addison's disease;
Various tumours are as substrate epithelial tumor, squama shape epithelial tumor, mucinous tumors, fibroma, lipoma, chondroma, vascular tumor, lymphoma, hemopoietic tissue tumour, neuroma, adenoma;
The present invention also provides SCREENED COMPOUND to identify the method that improves (agonist) or check the medicament of (antagonist) human glutaminyl tRNA synthetic enzyme 23.76.Agonist improves human glutaminyl tRNA synthetic enzyme 23.76 biological function such as stimulate cellular proliferation, and antagonist prevention disorder such as the various cancer relevant with cell hyperproliferation with treatment.For example, can in the presence of medicine, the film preparation of mammalian cell or expressing human glutamy tRNA synthetic enzyme 23.76 be cultivated with the human glutaminyl tRNA synthetic enzyme 23.76 of mark.Measure the medicine raising then or check this interactional ability.
The antagonist of human glutaminyl tRNA synthetic enzyme 23.76 comprises antibody, compound, acceptor disappearance thing and the analogue etc. that filter out.The antagonist of human glutaminyl tRNA synthetic enzyme 23.76 can combine and eliminate its function with human glutaminyl tRNA synthetic enzyme 23.76, or suppresses the generation of this polypeptide, or combines with the avtive spot of this polypeptide and to make this polypeptide can not bring into play biological function.
In screening during as the compound of antagonist, human glutaminyl tRNA synthetic enzyme 23.76 can be added in the bioanalysis mensuration, interactional influence between human glutaminyl tRNA synthetic enzyme 23.76 and its acceptor be determined whether compound is antagonist by measuring compound.With the same quadrat method of above-mentioned SCREENED COMPOUND, can filter out the acceptor disappearance thing and the analogue of antagonist action.Can be incorporated into the rondom polypeptide storehouse that solid formation forms by the various amino acid that may make up by screening with human glutaminyl tRNA synthetic enzyme 23.76 bonded peptide molecules obtains.During screening, generally tackle human glutaminyl tRNA synthetic enzyme 23.76 molecules and carry out mark.
The invention provides and use polypeptide, and fragment, derivative, analogue or their cell are as the method for antigen with production antibody.These antibody can be polyclonal antibody or monoclonal antibody.The present invention also provides the antibody at human glutaminyl tRNA synthetic enzyme 23.76 antigenic determinants.These antibody include, but is not limited to: the fragment that polyclonal antibody, monoclonal antibody, chimeric antibody, single-chain antibody, Fab fragment and Fab expression library produce.
The method of the available human glutaminyl tRNA of the production of polyclonal antibody synthetic enzyme 23.76 direct injection immune animals (as rabbit, mouse, rat etc.) obtains, and multiple adjuvant can be used for the enhancing immunity reaction, includes but not limited to freund's adjuvant etc.The technology of the monoclonal antibody of preparation human glutaminyl tRNA synthetic enzyme 23.76 includes but not limited to hybridoma technology (Kohler and Milstein.Nature, 1975,256:495-497), three knurl technology, people B-quadroma technology, EBV-hybridoma technology etc.With the variable region bonded chimeric antibody in human constant region and inhuman source can with existing technology production (Morrison et al, PNAS, 1985,81:6851).And the technology of existing manufacture order chain antibody (U.S.Pat No.4946778) also can be used for producing the single-chain antibody of anti-human glutaminyl tRNA synthetic enzyme 23.76.
The antibody of anti-human glutaminyl tRNA synthetic enzyme 23.76 can be used in the immunohistochemistry technology, detects the human glutaminyl tRNA synthetic enzyme 23.76 in the biopsy specimen.
With the also available labelled with radioisotope of human glutaminyl tRNA synthetic enzyme 23.76 bonded monoclonal antibodies, inject in the body and can follow the tracks of its position and distribution.This radiolabeled antibody can be used as a kind of atraumatic diagnostic method and is used for the location of tumour cell and has judged whether transfer.
Antibody also can be used for designing the immunotoxin at a certain privileged sites in the body.As the monoclonal antibody of human glutaminyl tRNA synthetic enzyme 23.76 high-affinities can with bacterium or plant poison (as diphtheria toxin, ricin, abrine etc.) covalent attachment.A kind of usual method is with sulfydryl linking agent such as SPDP, attacks the amino of antibody, by the exchange of disulfide linkage, toxin is incorporated on the antibody, and this hybrid antibody can be used for killing human glutaminyl tRNA synthetic enzyme 23.76 positive cells.
The disease that antibody among the present invention can be used for treating or prevention and human glutaminyl tRNA synthetic enzyme 23.76 are relevant.The antibody that gives suitable dosage can stimulate or block the generation or the activity of human glutaminyl tRNA synthetic enzyme 23.76.
The invention still further relates to the diagnostic testing process of quantitative and detection and localization human glutaminyl tRNA synthetic enzyme 23.76 levels.These tests are known in the art, and comprise that FISH measures and radioimmunoassay.Human glutaminyl tRNA synthetic enzyme 23.76 levels that detected in the test can be with laying down a definition the importance of human glutaminyl tRNA synthetic enzyme 23.76 in various diseases and be used to the disease of diagnosing human glutaminyl tRNA synthetic enzyme 23.76 to work.
Polypeptide of the present invention also can be used as the peptide spectrum analysis, for example, the polypeptide available physical, chemistry or enzyme carry out the specificity cutting, and carries out the two-dimentional or three-dimensional gel electrophoresis analysis of one dimension, be more preferably and carry out mass spectroscopy.
The polynucleotide of coding human glutaminyl tRNA synthetic enzyme 23.76 also can be used for multiple therapeutic purpose.Gene therapy technology can be used for treating because cell proliferation, growth or the metabolic disturbance due to the nothing expression of human glutaminyl tRNA synthetic enzyme 23.76 or the unusual/non-activity expression.The gene therapy vector (as virus vector) of reorganization can be designed for the human glutaminyl tRNA synthetic enzyme 23.76 of expressing variation, to suppress endogenic human glutaminyl tRNA synthetic enzyme 23.76 activity.For example, a kind of human glutaminyl tRNA synthetic enzyme 23.76 of variation can be the human glutaminyl tRNA synthetic enzyme 23.76 that shortens, lacked signal conduction function territory, though can combine with the substrate in downstream, lacks signaling activity.Therefore the gene therapy vector of reorganization can be used for treating the disease of 23.76 expression of human glutaminyl tRNA synthetic enzyme or active caused by abnormal.Deriving from viral expression vector such as retrovirus, adenovirus, adeno-associated virus (AAV), hsv, parvovirus etc. can be used for the polynucleotide of coding human glutaminyl tRNA synthetic enzyme 23.76 are transferred in the cell.The method of recombinant viral vector that structure carries the polynucleotide of coding human glutaminyl tRNA synthetic enzyme 23.76 is found in existing document (Sambrook, et al.).The polynucleotide of reorganization coding human glutaminyl tRNA synthetic enzyme 23.76 can be packaged in the liposome and be transferred in the cell in addition.
Polynucleotide import tissue or intracellular method comprises: directly be injected into polynucleotide in the in-vivo tissue; Or external by carrier (as virus, phage or plasmid etc.) earlier with the polynucleotide transfered cell in, again cell is transplanted in the body etc.
Suppress the oligonucleotide (comprising sense-rna and DNA) of human glutaminyl tRNA synthetic enzyme 23.76 mRNA and ribozyme also within the scope of the invention.Ribozyme is the enzyme sample RNA molecule that a kind of energy specificity is decomposed specific RNA, and its mechanism of action is to carry out the endonuclease effect after ribozyme molecule and the hybridization of complementary target RNA-specific.The RNA of antisense and DNA and ribozyme can obtain with existing any RNA or DNA synthetic technology, as the technology widespread use of solid phase phosphoamide chemical synthesis synthetic oligonucleotide.Antisense rna molecule can be transcribed acquisition by the dna sequence dna of this RNA that encodes in external or body.This dna sequence dna has been incorporated into the downstream of rna polymerase promoter of carrier.In order to increase the stability of nucleic acid molecule, available several different methods is modified it, and as increasing the sequence length of both sides, the connection between the ribonucleoside is used phosphoric acid thioester bond or peptide bond but not phosphodiester bond.
The polynucleotide of coding human glutaminyl tRNA synthetic enzyme 23.76 can be used for the diagnosis with the relative disease of human glutaminyl tRNA synthetic enzyme 23.76.The unconventionality expression of the expression that the polynucleotide of coding human glutaminyl tRNA synthetic enzyme 23.76 can be used for detecting human glutaminyl tRNA synthetic enzyme 23.76 human glutaminyl tRNA synthetic enzyme 23.76 whether or under morbid state.As the dna sequence dna of the human glutaminyl tRNA synthetic enzyme 23.76 of encoding can be used for biopsy specimen is hybridized to judge the expression situation of human glutaminyl tRNA synthetic enzyme 23.76.Hybridization technique comprises the Southern blotting, Northern blotting, in situ hybridization etc.These technological methods all are disclosed mature technologies, and relevant test kit all can obtain from commercial channels.Part or all of polynucleotide of the present invention can be used as probe stationary on microarray (Microarray) or DNA chip (being called " gene chip " again), is used for analyzing the differential expression analysis and the gene diagnosis of tissue gene.Carry out the transcription product that RNA-polymerase chain reaction (RT-PCR) amplification in vitro also can detect human glutaminyl tRNA synthetic enzyme 23.76 with human glutaminyl tRNA synthetic enzyme 23.76 special primers.
The sudden change that detects human glutaminyl tRNA synthetic enzyme 23.76 genes also can be used for diagnosing the relevant disease of human glutaminyl tRNA synthetic enzyme 23.76.The form of human glutaminyl tRNA synthetic enzyme 23.76 sudden change comprises that the point mutation compared with normal wild type human glutaminyl tRNA synthetic enzyme 23.76 dna sequence dnas, transposition, disappearance, reorganization and other are any unusual etc.Available existing technology such as Southern blotting, dna sequence analysis, PCR and in situ hybridization detect sudden change.In addition, sudden change might influence proteic expression, therefore can judge indirectly that with Northern blotting, Western blotting gene has or not sudden change.
Sequence of the present invention identifies it also is valuable to karyomit(e).This sequence can be specifically at certain bar human chromosome particular location and and can with its hybridization.At present, need to identify the concrete site of each gene on the karyomit(e).Now, have only chromosomal marker thing seldom to can be used for the marker chromosomes position based on actual sequence data (repetition polymorphism).According to the present invention, for these sequences are associated with disease related gene, its important the first step is positioned these dna sequence dnas on the karyomit(e) exactly.
In brief, prepare PCR primer (preferred 15-35bp), sequence can be positioned on the karyomit(e) according to cDNA.Then, these primers are used for the somatocyte hybrid cell that the PCR screening contains each bar human chromosome.Have only those hybrid cells that contain corresponding to the people's gene of primer can produce the fragment of amplification.
The PCR localization method of somatocyte hybrid cell is that DNA is navigated to concrete chromosomal quick method.Use Oligonucleolide primers of the present invention,, can utilize one group to realize inferior location from specific chromosomal fragment or a large amount of genomic clone by similar approach.Other the similar strategy that can be used for chromosomal localization comprises in situ hybridization, uses the karyomit(e) prescreen and the hybridization preliminary election of the airflow classification of mark, thereby makes up the special cDNA storehouse of karyomit(e).
The cDNA clone is carried out fluorescence in situ hybridization (FISH) with Metaphase Chromosome, can in a step, accurately carry out chromosomal localization.The summary of this technology is referring to Verma etc., Human Chromosomes:a Manualof Basic Techniques, Pergamon Press, New York (1988).
In case sequence is positioned to chromosome position accurately, the physical location of this sequence on karyomit(e) just can be associated with the gene map data.These data for example are found in, V.Mckusick, MendelianInheritance in Man (can by with the online acquisition of Johns Hopkins University Welch Medical Library).Can pass through linkage analysis then, determine gene and navigated to relation between the disease on the chromosomal region already.
Then, need to measure ill and not cDNA between diseased individuals or genome sequence difference.If observe certain sudden change in some or all of diseased individuals, and this sudden change is not observed in any normal individual, then this sudden change may be the cause of disease of disease.More ill and diseased individuals not is usually directed at first seek the variation of structure in the karyomit(e), as from the horizontal visible of karyomit(e) or use based on detectable disappearance of the PCR of cDNA sequence or transposition.Resolving power according to present physical mapping and assignment of genes gene mapping technology, being accurately positioned to the cDNA of the chromosomal region relevant with disease, can be a kind of (the supposing that 1 megabasse mapping resolving power and every 20kb are corresponding to a gene) between 50 to 500 potential Disease-causing genes.
Polypeptide of the present invention, polynucleotide and stand-in thereof, agonist, antagonist and inhibitor and suitable pharmaceutical carrier combination back can be used.These carriers can be water, glucose, ethanol, salt, damping fluid, glycerine and their combination.Composition comprises the polypeptide or the antagonist of safe and effective amount and carrier and the vehicle that does not influence effect of drugs.These compositions can be used as medicine and are used for disease treatment.
The present invention also provides medicine box or the test kit that contains one or more containers, and one or more medicinal compositions compositions of the present invention are housed in the container.With these containers, can have by the given indicative prompting of government authorities of making, using or selling medicine or biological products, the government authorities that this prompting reflects production, uses or sells permits it to use on human body.In addition, polypeptide of the present invention can be used in combination with other treatment compound.
Pharmaceutical composition can be with mode administration easily, as by in part, intravenously, intraperitoneal, intramuscular, subcutaneous, the nose or the route of administration of intracutaneous.Human glutaminyl tRNA synthetic enzyme 23.76 comes administration with the amount that treats and/or prevents concrete indication effectively.The amount and the dosage range that are applied to patient's human glutaminyl tRNA synthetic enzyme 23.76 will depend on many factors, as administering mode, person's to be treated healthiness condition and diagnostician's judgement.
Following accompanying drawing is used to illustrate specific embodiments of the present invention, and is not used in qualification by the scope of the invention that claims defined.
Fig. 1 is the gene chip expression spectral comparison diagram of inventor's glutamy tRNA synthetic enzyme 23.76 and human glutaminyl tRNA synthetic enzyme.Last figure is the express spectra folding side figure of human glutaminyl tRNA synthetic enzyme 23.76, and the below sequence is the express spectra folding side figure of human glutaminyl tRNA synthetic enzyme.Wherein, 1-tire brain, 2-normal brain activity, 3-tire kidney, 4-liver cancer, 5-tire liver, 6-adult liver, 7-Tiroidina, 8-tire lung, 9-lung, 10-muscle, 11-thymus gland, 12-glioma.
Fig. 2 is the polyacrylamide gel electrophoresis figure (SDS-PAGE) of isolating human glutaminyl tRNA synthetic enzyme 23.76.23.76kDa be proteinic molecular weight.The arrow indication is isolated protein band.
Below in conjunction with specific embodiment, further set forth the present invention.Should be understood that these embodiment only to be used to the present invention is described and be not used in and limit the scope of the invention.The experimental technique of unreceipted actual conditions in the following example, usually according to people such as normal condition such as Sambrook, molecular cloning: laboratory manual (New York:ColdSpring Harbor Laboratory Press, 1989) condition described in, or the condition of advising according to manufacturer.Embodiment 1: the clone of human glutaminyl tRNA synthetic enzyme 23.76
Extract the total RNA of people's tire brain with guanidinium isothiocyanate/phenol/chloroform single stage method.From total RNA, separate poly (A) mRNA with Quik mRNA Isolation Kit (Qiegene company product).2ug poly (A) mRNA forms cDNA through reverse transcription.CDNA fragment orientation is inserted on the multiple clone site of pBSK (+) carrier (Clontech company product) with Smart cDNA clone's test kit (available from Clontech), transforms DH5 α, bacterium forms the cDNA library.Measure all clones' 5 ' and 3 ' terminal sequence with Dyeterminate cycle reaction sequencing kit (Perkin-Elmer company product) and ABI 377 automatic sequencers (Perkin-Elmer company).CDNA sequence and the existing public dna sequence data storehouse (Genebank) measured are compared, found that the cDNA sequence of one of them clone 1734c01 is new DNA.By synthetic a series of primers the contained insertion cDNA fragment of this clone is carried out two-way mensuration.The result shows, the contained full-length cDNA of 1734c01 clone is 4070bp (shown in Seq ID NO:1), from 83bp to 733bp the open reading frame (ORF) of a 651bp, the new protein (shown in SeqID NO:2) of encoding arranged.We are with this clone's called after pBS-1734c01, encoded protein matter called after human glutaminyl tRNA synthetic enzyme 23.76.Embodiment 2: with the gene of RT-PCR method clones coding human glutaminyl tRNA synthetic enzyme 23.76
Total RNA is a template with fetus brain cell, is that primer carries out the synthetic cDNA of reverse transcription reaction with oligo-dT, with behind the test kit purifying of Qiagene, carries out pcr amplification with following primer:
Primer1:5’-GCCGGCGGCTCCGCTTTCCCGGCT-3’(SEQ?ID?NO:3)
Primer2:5’-CATAGGCCGAGGCGGCCGACATGT-3’(SEQ?ID?NO:4)
Primer1 is the forward sequence that begins of 1bp that is positioned at the 5 ' end of SEQ ID NO:1;
Primer2 be SEQ ID NO:1 in 3 ' end reverse sequence.
The condition of amplified reaction: in the reaction volume of 50 μ l, contain 50mmol/L KCl, 10mmol/L Tris-Cl, (pH8.5), 1.5mmol/L MgCl
2, 200 μ mol/L dNTP, 10pmol primer, the Taq archaeal dna polymerase of 1U (Clontech company product).Go up by 25 cycles of following conditioned response at PE9600 type DNA thermal cycler (Perkin-Elmer company): 94 ℃ of 30sec; 55 ℃ of 30sec; 72 ℃ of 2min.When RT-PCR, establish the blank negative contrast of positive contrast of β-actin and template simultaneously.Amplified production is connected to (Invitrogen company product) on the pCR carrier with the test kit purifying of QIAGEN company with TA clone test kit.The dna sequence analysis result shows that the dna sequence dna of PCR product and the 1-4070bp shown in the SEQ ID NO:1 are identical.Embodiment 3:Northern blotting analyst glutamy tRNA synthetic enzyme 23.76 expression of gene:
Extract total RNA[Anal.Biochem 1987,162,156-159 with single stage method].This method comprises acid guanidine thiocyanate phenol-chloroform extracting.Promptly use 4M guanidinium isothiocyanate-25mM Trisodium Citrate, 0.2M sodium acetate (pH4.0) carries out homogenate to tissue, adds the phenol of 1 times of volume and the chloroform-primary isoamyl alcohol (49: 1) of 1/5 volume, and is centrifugal after mixing.The sucking-off aqueous phase layer adds Virahol (0.8 volume) and with the centrifugal RNA precipitation that obtains of mixture.With RNA precipitation 70% washing with alcohol that obtains, dry and soluble in water.With 20 μ g RNA, on 1.2% sepharose that contains 20mM 3-(N-morpholino) propanesulfonic acid (pH7.0)-5mM sodium acetate-1mM EDTA-2.2M formaldehyde, carry out electrophoresis.Be transferred on the nitrocellulose filter then.With α-
32P dATP prepares by random priming
32The dna probe of P-mark.Used dna probe is human glutaminyl tRNA synthetic enzyme 23.76 coding region sequences (83bp to 733bp) of pcr amplification shown in Figure 1.Probe (about 2 * 10 with the 32P-mark
6Cpm/ml) spend the night in 42 ℃ of hybridization in a solution with the nitrocellulose filter that has shifted RNA, this solution comprises 50% methane amide-25mM KH
2PO
4(pH7.4)-5 * SSC-5 * Denhardt ' s solution and 200 μ g/ml salmon sperm DNAs.After the hybridization, filter membrane is washed 30min in 55 ℃ in 1 * SSC-0.1%SDS.Then, analyze with quantitative with Phosphor Imager.Embodiment 4: vivoexpression, separation and the purifying of recombinant human glutamy tRNA synthetic enzyme 23.76
According to SEQ ID NO:1 and coding region sequence shown in Figure 1, design a pair of specificity amplification primer, sequence is as follows:
Primer3:5’-CATGCTAGCATGAACAGCGGCGGCGGCTTCGGT-3’(Seq?ID?No:5)
Primer4:5’-CCCGAGCTCTTATTCTGCCATCCGCACAAACTT-3’(Seq?ID?No:6)
5 ' end of these two sections primers contains NheI and SacI restriction enzyme site respectively, be respectively the encoding sequence of target gene 5 ' end and 3 ' end thereafter, NheI and SacI restriction enzyme site are corresponding to expression vector plasmid pET-28b (+) (Novagen company product, Cat.No.69865.3) the selectivity restriction enzyme site on.With the pBS-1734c01 plasmid that contains the total length goal gene is template, carries out the PCR reaction.The PCR reaction conditions is: contain pBS-1734c01 plasmid 10pg, primer Primer-3 and Primer-4 among the cumulative volume 50 μ l and be respectively 10pmol, Advantage polymerase Mix (Clontech company product) 1 μ l.Loop parameter: 94 ℃ of 20s, 60 ℃ of 30s, 68 ℃ of 2min, totally 25 circulations.Respectively amplified production and plasmid pET-28 (+) are carried out double digestion with NheI and SacI, reclaim big fragment respectively, and connect with the T4 ligase enzyme.Connect product and transform, after the dull and stereotyped overnight incubation of the LB that contains kantlex (final concentration 30 μ g/ml), use the colony polymerase chain reaction (PCR) method screening positive clone, and check order with the big enterobacterial DH5 of Calcium Chloride Method α.Select the correct positive colony of sequence (pET-1734c01) with Calcium Chloride Method with recombinant plasmid transformed e. coli bl21 (DE3) plySs (Novagen company product).In the LB liquid nutrient medium that contains kantlex (final concentration 30 μ g/ml), host bacterium BL21 (pET-1734c01) is cultured to logarithmic phase at 37 ℃, adds IPTG to final concentration 1mmol/L, continues to cultivate 5 hours.Centrifugal collection thalline, through the broken bacterium of ultrasonic wave, centrifugal collection supernatant with carrying out chromatography with 6 Histidines (6His-Tag) bonded affinity column His.Bind Quick Cartridge (Novagen company product), has obtained the target protein human glutaminyl tRNA synthetic enzyme 23.76 of purifying.Through the SDS-PAGE electrophoresis, obtain a single band (Fig. 2) at the 23.76kDa place.This band is transferred on the pvdf membrane carries out the n terminal amino acid sequential analysis with the Edams hydrolysis method, 15 amino acid of N-end hold 15 amino-acid residues identical with the N-shown in the SEQ ID NO:2 as a result.Embodiment 5 anti-human glutaminyl tRNA synthetic enzyme 23.76 production of antibodies
Synthesize following human glutaminyl tRNA synthetic enzyme 23.76 specific polypeptide with Peptide synthesizer (PE company product):
NH2-Met-Asn-Ser-Gly-Gly-Gly-Phe-Gly-Leu-Gly-Leu-Gly-Phe-Gly-Leu-COOH(SEQ?ID?NO:7)。Form compoundly with hemocyanin and bovine serum albumin coupling this polypeptide respectively, method is referring to Avrameas, et al.Immunochemistry, 1969; 6:43.Add the complete Freund's adjuvant immunizing rabbit with the above-mentioned hemocyanin polypeptide complex of 4mg, add the incomplete Freund's adjuvant booster immunization once with the hemocyanin polypeptide complex again after 15 days.Employing is done the titre that ELISA measures antibody in the rabbit anteserum through the titer plate of 15 μ g/ml bovine serum albumin polypeptide complex bag quilts.From the rabbit anteserum of antibody positive, separate total IgG with albumin A-Sepharose.Polypeptide is incorporated on the Sepharose4B post of cyanogen bromide-activated, from total IgG, separates anti-peptide antibody with affinity chromatography.Immuno-precipitation proof antibody purified can combine with human glutaminyl tRNA synthetic enzyme 23.76 specifically.Embodiment 6: polynucleotide passage of the present invention is as the application of hybridization probe
Picking out suitable oligonucleotide fragment from polynucleotide of the present invention is of use in many ways as hybridization probe, as can whether containing polynucleotide sequence of the present invention and detect the homologous polynucleotide sequence to identify it with the healthy tissues of different sources or the genome or the hybridization of cDNA library of pathological tissue with this probe, whether further also available this probe in detecting polynucleotide sequence of the present invention or the expression of its homologous polynucleotide sequence in healthy tissues or pathological tissue cell be unusual.
The purpose of present embodiment is to pick out suitable oligonucleotide fragment as hybridization probe from polynucleotide SEQ ID NO:1 of the present invention, and identifies in some tissues whether contain polynucleotide sequence of the present invention or its homologous polynucleotide sequence with the filter hybridization method.The filter hybridization method comprises dot blotting, Southern blotting, Northern blotting and copy method etc., and they all are that polynucleotide sample to be measured is fixed on use essentially identical step crossover in back on the filter membrane.These identical steps are: the filter membrane of having fixed sample at first carries out prehybridization with the hybridization buffer that does not contain probe, so that nonspecific combining site suppressed by vector of sample and synthetic polymer institute are saturated on the filter membrane.Prehybridization solution is contained the hybridization buffer replacement of label probe then, and insulation makes probe and target nucleic acid hybridization.After the hybridization step, the probe in the hybridization is not removed by a series of film steps of washing.Present embodiment utilizes the film condition of washing (as than low salt concn and higher temperature) of higher-strength, so that hybrid context reduces and only keep the signal of high specificity.The probe that present embodiment is selected for use comprises two classes: first kind probe be fully with the identical or complementary oligonucleotide fragment of polynucleotide SEQ ID NO:1 of the present invention; The second class probe is part and the identical or complementary oligonucleotide fragment of polynucleotide SEQ ID NO:1 of the present invention.Present embodiment selects for use dot blotting that sample is fixed on the filter membrane, higher-strength wash under the film condition, the hybridization specificity of first kind probe and sample is the strongest and kept.One, probe selects for use
From polynucleotide SEQ ID NO:1 of the present invention, select oligonucleotide fragment as hybridization probe, the several aspects that should follow following principle and need to consider: 1, the probe size preferable range is a 18-50 Nucleotide; 2, GC content is 30%-70%, and surpassing then, non-specific hybridization increases; 3, probe interior should not have complementary region; 4, what meet above condition can be used as the primary election probe, further do the computer sequential analysis then, comprise this primary election probe is carried out homology relatively with its source sequence area (being SEQ ID NO:1) and other known genome sequence and complementary district thereof respectively, if with the homology in non-target molecule zone greater than 85% or there are 15 continuous bases of surpassing identical, then this primary election probe is general just should not use; 5, whether the primary election probe finally is chosen to be the probe of actual application value also should further be determined by experiment.Select and synthetic following two probes after finishing the analysis of above each side:
Probe 1 (probe1) belongs to first kind probe, and complete homology of gene fragment or the complementation (41Nt) of SEQ ID NO:1:
5’-TGAACAGCGGCGGCGGCTTCGGTTTGGGCTTAGGCTTCGGC-3’(SEQ?ID?NO:8)
Probe 2 (probe2) belongs to the second class probe, is equivalent to gene fragment or its complementary segmental replacement mutant nucleotide sequence (41Nt) of SEQ ID NO:1:
5’-TGAACAGCGGCGGCGGCTTCAGTTTGGGCTTAGGCTTCGGC-3’(SEQ?ID?NO:9)
Other unlisted common agents and the compound method thereof relevant with following concrete experimental procedure please refer to document: DNA PROBES G.H.Keller; M.M.Manak; Stockton Press, 1989 (USA) and molecular cloning laboratory manual books more commonly used are as works such as " molecular cloning experiment guide " (second edition in 1998) [U.S.] Sa nurse Brooker, Science Press.
Specimen preparation: 1, from fresh or frozen tissue, extract DNA
Step: 1) the fresh or fresh normal liver tissue that thaws is put into the plate that is immersed on ice and fills phosphate buffered saline buffer (PBS).With scissors or scalpel tissue is cut into small pieces.Should keep organizing moistening in the operation.2) with 1000g centrifugal chopper tissue 10 minutes.3) with cooled homogenate damping fluid (0.25mol/L sucrose; 25mmol/LTris-HCl, pH7.5; 25mmol/LnaCl; 25mmol/L MgCl
2) precipitation that suspends (approximately 10ml/g).4) 4 ℃ with electric homogenizer homogenate tissue suspension at full speed, until tissue by broken fully.5) 1000g is centrifugal 10 minutes.6) with re-suspended cell precipitation (the initial tissue sample of every 0.1g adds 1-5ml), centrifugal 10 minutes again with 1000g.7) with the resuspended precipitation of lysis buffer (the initial tissue sample of every 0.1g adds 1ml), connect following phenol extraction process then.2, the phenol extraction process of DNA
Step: 1) wash cell, centrifugal 10 minutes of 1000g with the cold PBS of 1-10ml.2) with the sedimentary cell (1 * 10 of cold cell pyrolysis liquid resuspension
8The minimum of applications 100ul lysis buffer of cell/ml).3) adding SDS is 1% to final concentration, if before re-suspended cell SDS is directly joined in the cell precipitation, cell may form big agglomerate and be difficult to fragmentation, and the overall yield that reduces.This point is in extracting>10
7Especially severe during cell.4) add Proteinase K to final concentration 200ug/ml.5) 50 ℃ of insulation reaction 1 hour or 37 ℃ gently jolting spend the night.6) use equal-volume phenol: chloroform: primary isoamyl alcohol (25: 24: 1) extracting, in little centrifuge tube centrifugal 10 minutes.Two corresponding clear separation, otherwise carry out centrifugal again.7) water is transferred to new pipe.8) use the equal-volume chloroform: primary isoamyl alcohol (24: 1) extracting, centrifugal 10 minutes.9) water that will contain DNA is transferred to new pipe.Carry out purifying and the ethanol sedimentation of DNA then.3, the purifying of DNA and ethanol sedimentation
Step: 1) 1/10 volume 2mol/L sodium-acetate and 2 times of cold 100% ethanol of volume are added in the dna solution mixing.-20 ℃ of placements 1 hour or to spending the night.2) centrifugal 10 minutes.3) careful sucking-off or pour out ethanol.4) with 70% cold ethanol 500ul washing precipitation, centrifugal 5 minutes.5) careful sucking-off or pour out ethanol.With the cold washing with alcohol precipitation of 500ul, centrifugal 5 minutes.6) careful sucking-off or pour out ethanol is inverted on thieving paper then residual ethanol is flow to end.Dry air 10-15 minute, so that the volatilization of surperficial ethanol.Note not making the precipitation complete drying, otherwise dissolve again than difficulty.7) with small volume TE or the resuspended DNA precipitation of water.The low speed vortex vibrates or uses the dropper pressure-vaccum, increases TE gradually simultaneously, is mixed to DNA and fully dissolves, every 1-5 * 10
6Cell extracted approximately adds 1ul.
Below the 8-13 step only be used for must removing when depolluting, otherwise can directly carry out the 14th step.8) RNA enzyme A is added in the dna solution, final concentration is 100ug/ml, and 37 ℃ are incubated 30 minutes.9) add SDS and Proteinase K, final concentration is respectively 0.5% and 100ug/ml.37 ℃ are incubated 30 minutes.10) use isopyknic phenol: chloroform: primary isoamyl alcohol (25: 24: 1) extractive reaction liquid, centrifugal 10 minutes.11) carefully shift out water, use isopyknic chloroform: primary isoamyl alcohol (24: 1) extracting again, centrifugal 10 minutes.12) carefully shift out water, add 1/10 volume 2mol/L sodium-acetate and the cold ethanol of 2.5 volumes, mixing put-20 ℃ 1 hour.13) with 70% ethanol and 100% washing with alcohol precipitation, dry air, resuspended nucleic acid, process is with the 3-6 step.14) measure A
260And A
280To detect purity and the productive rate of DNA.15) deposit in-20 ℃ after the packing.The preparation of sample film:
1) get 4 * 2 suitably nitrocellulose filters (NC film) of size, mark point sample position and sample number thereon gently with pencil, each probe needs two NC films, so that wash film with high strength condition and strength condition respectively in the experimental procedure of back.
2) draw and contrast respectively 15 microlitres, put on the sample film, dry at room temperature.
3) place infiltration that 0.1mol/LNaOH is arranged, last 5 minute of filter paper (twice) of 1.5mol/LNaCl, drying to place to soak into has 0.5mol/L Tris-HCl (pH7.0), last 5 minute of filter paper (twice) of 3mol/LNaCl, dries.
4) be sandwiched in the clean filter paper, wrap, 60-80 ℃ of vacuum-drying 2 hours with aluminium foil.
The mark of probe
1) 3 μ lProbe (0.1OD/10 μ l) add 2 μ lKinase damping fluids, 8-10uCi γ-
32P-dATP+2UKinase is to add to final volume 20 μ l.
2) 37 ℃ are incubated 2 hours.
3) add the tetrabromophenol sulfonphthalein indicator (BPB) of 1/5 volume.
4) cross Sephadex G-50 post.
5) to having
32Before washing out, P-Probe begins to collect first peak (available Monitor monitoring).
6) 5/pipe, collect the 10-15 pipe.
7) monitor isotopic weight with liquid glimmer instrument
8) merge and to be required preparation behind the collection liquid of first peak
32P-Probe (second peak for free γ-
32P-dATP).
Prehybridization
The sample film is placed plastics bag, and adding 3-10mg prehybridization solution (10 * Denhardt ' s; 6 * SSC, 0.1mg/mlCT DNA (calf thymus DNA).), seal sack after, 68 ℃ of water-baths were shaken 2 hours.
Hybridization
Plastics bag is cut off one jiao, adds the probe prepare, seal sack after, 42 ℃ of water-baths are shaken and are spent the night.
Wash film: high strength is washed film:
1) good sample film has been hybridized in taking-up.
2) 2 * SSC among the 0.1%SDS, washes 15 minutes (2 times) for 40 ℃.
3) 0.1 * SSC among the 0.1%SDS, washes 15 minutes (2 times) for 40 ℃.
4) 0.1 * SSC among the 0.1%SDS, washes 30 minutes (2 times) for 55 ℃, and room temperature is dried.Low strength is washed film:
1) good sample film has been hybridized in taking-up.
2) 2 * SSC among the 0.1%SDS, washes 15 minutes (2 times) for 37 ℃.
3) 0.1 * SSC among the 0.1%SDS, washes 15 minutes (2 times) for 37 ℃.
4) 0.1 * SSC among the 0.1%SDS, washes 15 minutes (2 times) for 40 ℃, and room temperature is dried.
X-light autography:
-70 ℃, X-light autography (the compressing tablet time decides according to hybridization spot radioactivity is strong and weak).
Experimental result:
Adopt low strength to wash the hybrid experiment that the film condition is carried out, more than two strong and weak not obviously differences of probe hybridization spot radioactivity; And adopting high strength to wash the hybrid experiment that the film condition is carried out, the hybridization spot radioactive intensity of probe 1 obviously is better than the radioactive intensity of another probe hybridization spot.Thereby available probe 1 is qualitative and analyze existence and the differential expression of polynucleotide of the present invention in different tissues quantitatively.Embodiment 7 DNA Microarray
Gene chip or gene micromatrix (DNA Microarray) are that present many National Laboratories and big drugmaker are all in the new technology of setting about developing and developing, it is meant and is arranged in a large amount of target fragments on the carriers such as glass, silicon in an orderly manner, to high-density, carry out the comparison and the analysis of data then with fluoroscopic examination and computer software, to reach purpose quick, efficient, that bioinformation is analyzed on high-throughput ground.Polynucleotide of the present invention can be used as target DNA and are used for biochip technology and are used for high-throughput and study new gene function; Seek and the new gene of the screening tissue specificity new gene of disease-related such as tumour particularly; The diagnosis of disease is as heredopathia.The existing in the literature multiple report of its concrete grammar step is as consulting document DeRisi, J.L., Lyer, V.﹠amp; Brown, P.O. (1997) Science278,680-686. and document Helle, R.A., Schema, M., Chai, A., Shalom, D., (1997) PNAS 94:2150-2155. () point sample
Various full-length cDNA amounts to 4000 polynucleotide sequences as target DNA, comprising polynucleotide of the present invention.They are increased by PCR respectively, behind the purifying gained amplified production its concentration is transferred to about 500ng/ul, (available from U.S. Cartesian company) puts on glass medium with Cartesian 7500 point sample instruments, and distance between points is 280 μ m.Slide behind the point sample is carried out hydration, drying, places UV-crosslinked instrument crosslinked, and the wash-out after drying is fixed on DNA and is prepared into chip on the sheet glass.The existing in the literature multiple report of its concrete grammar step, the point sample post-processing step of present embodiment is:
1. hydration 4 hours in the wet environment;
2. the 0.2%SDS washing is 1 minute;
3.ddH
2The O washed twice, each 1 minute;
4.NaBH
4Sealed 5 minutes;
5. in 95 ℃ of water 2 minutes;
6. the 0.2%SDS washing is 1 minute;
7.ddH
2Twice of O flushing;
8. airing, 25 ℃ to be stored in the dark place standby.(2) probe mark
With the single stage method total mRNA of extracting from human body mixed structure and body particular organization (or through stimulated cells strain) respectively, and with Oligotex mRNA Midi Kit (available from QiaGen company) purified mRNA, by reverse transcription respectively with fluorescent reagent Cy3dUTP (5-Amino-propargyl-2 '-deoxyuridine 5 '-triphatecoupled to Cy3 fluorescent dye, available from Amersham Phamacia Biotech company) mRNA of mark human body mixed structure, with fluorescent reagent Cy5dUTP (5-Amino-propargyl-2 '-deoxyuridine5 '-triphate coupled to Cy5 fluorescent dye, available from Amersham Phamacia Biotech company) mRNA of mark body particular organization (or through stimulated cells strain), prepare probe after purified.Concrete steps reference and method are seen: Schena, M., Shalon, D., Heller, R. (1996) Proc.Natl.Acad.Sci.USA.Vol.93:10614-10619.Schena, M., Shalon, Dari., Davis, R.W. (1995) Science.270. (20): 467-480. (three) hybridization
Respectively will be from the probe of above two kinds of tissues with chip at UniHyb
TMHybridized 16 hours in HybridizationSolution (available from the TeleChem company) hybridization solution, room temperature washings (1 * SSC, 0.2%SDS) the washing back is scanned with ScanArray 3000 scanners (available from U.S. General Scanning company), the image of scanning carries out data analysis with Imagene software (U.S. Biodiscovery company) to be handled, and calculates the Cy3/Cy5 ratio of each point.
Be respectively normal brain activity, liver cancer, muscle, tire brain, tire kidney, tire lung, tire liver, Tiroidina, thymus gland, adult liver, lung, glioma with upper machine body particular organization (or through stimulated cells strain).Draw folding side figure according to these 12 Cy3/Cy5 ratios.(Fig. 1).Human glutaminyl tRNA synthetic enzyme 23.76 of the present invention as seen from the figure is very similar with human glutaminyl tRNA synthetic enzyme express spectra.
Sequence table (1) general information: (ii) denomination of invention: human glutaminyl tRNA synthetic enzyme 23.76 and encoding sequence thereof be the sequence number (iii): the information of 9 (2) SEQ ID NO:1: (i) sequence signature:
(A) length: 4070bp
(B) type: nucleic acid
(C) chain: two strands
( D ) : ( ii ) :cDNA ( xi ) :SEQ ID NO:1: 1 GCCGGCGGCTCCGCTTTCCCGGCTCCGTCGCTGACGCGTCGTAGACGTTGGGGAGCGGGA 61 AGGCAACGGCAGCGGGATCGGGATGAACAGCGGCGGCGGCTTCGGTTTGGGCTTAGGCTT121 CGGCCTCACCCCCACGTCGGTGATTCAGGTGACGAATCTGTCGTCGGCGGTGACCAGCGA181 GCAGATGCGGACGCTTTTTTCCTTCCTAGGAGAAATCGAGGAGCTGCGGCTCTACCCCCC241 GGACAACGCACCTCTTGCTTTTTCCTCCAAAGTATGTTATGTTAAGTTTCGTGATCCATC301 AAGTGTTGGCGTGGCCCAGCATCTAACTAACACGGTTTTTATTGACAGAGCTCTGATAGT361 TGTTCCTTGTGCAGAAGGTAAAATCCCAGAGGAATCCAAAGCCCTCTCTTTATTGGCTCC421 TGCTCCAACCATGACAAGTCTGATGCCTGGTGCAGGATTGCTTCCAATACCGACCCCAAA481 TCCTTTGACTACTCTTGGTGTTTCACTTAGCAGTTTGGGAGCTATACCAGCAGCAGCACT541 AGACCCCAACATTGCAACACTTGGAGAGATACCACAGCCACCACTTATGGGAAACGTGGA601 TCCTTCCAAAATAGATGAAATTAGGAGAACGGTTTATGTTGGAAATCTGAATTCCCAGAC661 AACGACAGCTGATCAACTACTTGAATTTTTTAAACAAGTTGGAGAAGTGAAGTTTGTGCG721 GATGGCAGAATAAATCACTCCAACAATGCAATAGTAAGACCCCCTGAGATGACACCTCAG781 GCTGCAGCTAAGGAGTTAGAAGAAGTAATGAAGCGAGTACGAGAAGCTCAGTCATTTATC841 TCAGCAGCTATTGAACCAGGGTGGCTGCACTCAACGAGTTTATGCAATGACTTTCTTGGA901 TGTTTCTGAAGGAGGAGGATGTACAGAGAGTAGGCCCCTTGCACTATATGTGGTACATTC 961 CACTTGTGCCTGATTATTAACTGGGATCTTTAATTGTTCTGAGCTTACACTGCAAAGTGA1021 TTTTTTCCTCCCAGAGTCTGGAAAGAGCAATGAAAGAAAAGGCGGTCGATCTCGTTCCCA1081 TACTCGCTCAAAATCCAGGTCTAGCTCAAAATCCCATTCTAGAAGGAAAAGATCACAATC1141 AAAACACAGGAGTAGATCCCATAATAGATCACGTTCAAGACAGAAAGACAGACGTAGATC1201 TAAGAGCCCACATAAAAAACGCTCTAAATCAAGGGAGAGACGGAAGTCAAGGAGTCGTTC1261 GCATTCACGGGACAAGAGAAAAGACACTCGAGAAAAGATCAAGGAAAAGGAAAGAGTGAA1321 AGAGAAAGACAGGGAAAAGGAGAGAGAGAGGGAAAAGGAACGTGAAAAAGAAAAGGAACG1381 GGGTAAAAACAAAGACCGGGACAAGGAACGGGAAAAGGACCGGGAAAAAGACAAGGAAAA1441 GGACAGAGAGAGAGAACGGGAAAAAGAGCATGAGAAGGATCGAGACAAAGAGAAGGAAAA1501 GGAACAGGACAAAGAAAAGGAACGAGAAAAAGACAGATCCAAAGAGATAGATGAAAAAAG1561 AAAGAAGGATAAAAAATCCAGAACACCACCCAGGAGTTACAATGCATCGCGAAGATCTCG1621 TAGTTCCAGCAGGGAAAGGCGTAGGAGGAGGAGCAGGAGTTCTTCCAGATCGCCAAGAAC1681 ATCAAAAACCATAAAAAGGAAATCTTCTAGATCTCCGTCCCCCAGGAGAAATAGGAAGGA1741 TAAAAAGAGAGAAAAAGAAAGGGACCACATCAGTGAAAGAAGAGAGAGAGAACGTTCAAC1801 GTCTATGAGAAAGAGTTCTAATGATAGAGATGGGAAGGAGAAGTTGGAGAAGAACAGTAC1861 TTCACTTAAAGAGAAAGAGCACAATAAAGAACCAGATTCAAGTGTGAGCAAAGAAGTAGA1921 TGACAAGGATGCACCAAGGACTGAGGAAAACAAAATACAGCACAATGGGAATTGTCAGCT1981 GAATGAAGAAAACCTCTCTACCAAAACAGAAGCAGTATAGGACCGACAAGTGTACCTCTG2041 CACTCAATGCTGGAATCAAATCCAAAGCTTTTAATTCTCTCAACAAGATGTAAACAGGAA2101 AGAAATCTAGTTGAGCATGAAGATAGGATCTAACAGCTTTTCCAGTTGTTAGATGACTTT2161 GTGGCCATCTTGTTATTGAGTAAGAAAATAAAGCATGGACATCATGAAAATAACAGATGT2221 TACCCAAACTCATCTTCTAAAATCTGTGCATTTCCATGGTGGCTGACACACTTGTCATGT2281 GGTCTGTTAGTGTTTGCCAAGAACCATTGCAAATAAATTGAACATCAAAGATCCAAGTTT2341 GTACTATCCCTAAAGACTGGAGATAAGCATTGGAGGCTCTTTTAAAAAATGCTAGTTACT2401 GAATTTTGTATTGTTTTACTTTTTTTTTATTTCAATATATACAGTTTGATGATGTGCTTG2461 AAATTGGTGCAAATATATACACACCCTTGTAAGTGCAAAGTATGTAAGAAGTTTTAACAT2521 TTACTTCACAGGACTTGTGATTGTGTTAAATTCTCACTATTGTGTTTTCTTTTGCTCACT2581 GTTTAGGACAATTTTTCTTTAAAATAGTTTTGCAGATTAAAATTGCTTAAATAAGTGGAT2641 TAAAAAACTGACAATGCATGCTACTGTTCTCTTTCAAAAGGAAGAGCAACCGTGTTGAAT2701 ACTAATAATGATGAATTAGTATTCAGTGTTTAGAATCATTGGGACTACCCACAAAGTGAG2761 CATTTCTTTTTAAATTTTCTTGACATTTCCAAGCTTATTATGAATAATATTGCAGTGTGT2821 CTTGTCAGCTGTAGGTGGCAAAGGTGCCCTTATAAAAAAGGAAACTGGCTTTTCAAAATG2881 GGCTATGGGAGCACAAGCTGAAGCTTTAGTGCCTTCTACAATGTGGTATACTGTTTTCTA2941 GAATTTTATATGTGCTAGTCATTCTCAATTCATATGGAATCTAGATGGATATTTCATGCA3001 TACCCATAGAGAAGTGTGTAAGTGATATGTCAGAAGAGCTTCTTACTGATTTCACCTAAA3061 ATGAGAAGGAAGTCCTGTTTTCAAGAATGACATTAGAGTCATGCAGCTTTGGGACCATCA3121 GTTTTATACTGTGATAATTGAAAATGAAACATGTTCTTATTTTCCTTAAATTGAAGAAAA3181 CCCTTTAGTTGTCTACATTGGATGGCCTTATTACCTCTCAATCATCTTTTCATAAATGAT3241 GTGCAGAAATTGTACTTAAGGACTTAGGAGTATATGGGAGGTTATTGGTTTTATGTTTAA3301 GGATACGTTTACTTGAGTTTAAGATACAGGTCATCCATCATTCTTAGGCTCACTTTTTAC3361 AGAAAGTATGCAAATAGTAAAGTGACAGCACTGCTAATGTTTTTCCCCAGTACTATAACT3421 TGTGGTTTCTGAACTCATTATTGTTGTATTTCCAAAAAAGTAATACCTTTTAATTAGTGT3481 ATTAAAAGTTAAGTATAATTATTTTAATGCAATCTAATACAATCAGATTACTCAGTTGCC3541 TTACCTCATGGGAAGAGTTACTTTTTTAGATCTAAAAAGCTGAATAGCATGTTAGTTACT3601 TGGTTTCAACTTGAGTTTTCTTTTAATGTTAATAAGATTGAAACTTTAGTATTTAGTGGG3661 GAATGGAAAGAGTTGCCCTTGTTGCAAGTAATGAAGCCTGATTTGATTATGAAGCTGCTT3721 AATCACTCTTCATGTGTTCAGAATTACTGTTTTTTTGTTTGTTTTTCCTTTTTGTCACTG3781 TGTACATTAAAATTTTGGAAGATGCTTTACTATGTAAAGTATAGATGGTCATTTTAATCA3841 TTCAGCCACATACGGTTGGCTGGTAAACAGCTTATTCTGATACAAGAATGCTTGGGTGCA3901 TATGGAAAGATTGTGAAAGAGTGTGTCTTGCATCAACAGCTGTCTTATTTATGATATATA3961 AGTAGAAATAGAGCAAATGTTGGAATCTGTTATTTTTAGTACCATGTCTTTAATAAAGCT4021 AAGTATTTTAGAGCAAAAAAAAAAAAACATGTCGGCCGCCTCGGCCTATG ( 3 ) SEQ ID NO:2:
(i) sequence signature:
(A) length: 216 amino acid
(B) type: amino acid
(D) topological framework: linearity
(ii) molecule type: polypeptide
( xi ) :SEQ ID NO:2: 1 Met Asn Ser Gly Gly Gly Phe Gly Leu Gly Leu Gly Phe Gly Leu16 Thr Pro Thr Ser Val Ile Gln Val Thr Asn Leu Ser Ser Ala Val31 Thr Ser Glu Gln Met Arg Thr Leu Phe Ser Phe Leu Gly Glu Ile 46 Glu Glu Leu Arg Leu Tyr Pro Pro Asp Asn Ala Pro Leu Ala Phe 61 Ser Ser Lys Val Cys Tyr Val Lys Phe Arg Asp Pro Ser Ser Val 76 Gly Val Ala Gln His Leu Thr Asn Thr Val Phe Ile Asp Arg Ala 91 Leu Ile Val Val Pro Cys Ala Glu Gly Lys Ile Pro Glu Glu Ser106 Lys Ala Leu Ser Leu Leu Ala Pro Ala Pro Thr Met Thr Ser Leu121 Met Pro Gly Ala Gly Leu Leu Pro Ile Pro Thr Pro Asn Pro Leu136 Thr Thr Leu Gly Val Ser Leu Ser Ser Leu Gly Ala Ile Pro Ala151 Ala Ala Leu Asp Pro Asn Ile Ala Thr Leu Gly Glu Ile Pro Gln166 Pro Pro Leu Met Gly Asn Val Asp Pro Ser Lys Ile Asp Glu Ile181 Arg Arg Thr Val Tyr Val Gly Asn Leu Asn Ser Gln Thr Thr Thr196 Ala Asp Gln Leu Leu Glu Phe Phe Lys Gln Val Gly Glu Val Lys211 Phe Val Arg Met Ala Glu ( 4 ) SEQ ID NO:3
(i) sequence signature
(A) length: 24 bases
(B) type: nucleic acid
(C) chain: strand
(D) topological framework: linearity
(ii) molecule type: oligonucleotide
(xi) sequence description: the information of SEQ ID NO:3:GCCGGCGGCTCCGCTTTCCCGGCT 24 (5) SEQ ID NO:4
(i) sequence signature
(A) length: 24 bases
(B) type: nucleic acid
(C) chain: strand
(D) topological framework: linearity
(ii) molecule type: oligonucleotide
(xi) sequence description: the information of SEQ ID NO:4:CATAGGCCGAGGCGGCCGACATGT 24 (6) SEQ ID NO:5
(i) sequence signature
(A) length: 33 bases
(B) type: nucleic acid
(C) chain: strand
(D) topological framework: linearity
(ii) molecule type: oligonucleotide (xi) sequence description: the information of SEQ ID NO:5:CATGCTAGCATGAACAGCGGCGGCGGCTTCGGT 33 (7) SEQ ID NO:6
(i) sequence signature
(A) length: 33 bases
(B) type: nucleic acid
(C) chain: strand
(D) topological framework: linearity
(ii) molecule type: oligonucleotide (xi) sequence description: the information of SEQ ID NO:6:CCCGAGCTCTTATTCTGCCATCCGCACAAACTT 33 (8) SEQ ID NO:7:
(i) sequence signature:
(A) length: 15 amino acid
(B) type: amino acid
(D) topological framework: linearity
(ii) molecule type: polypeptide (xi) sequence description: the information of SEQ ID NO:7:Met-Asn-Ser-Gly-Gly-Gly-Phe-Gly-Leu-Gly-Leu-Gly-Phe-Gly-Leu 15 (9) SEQ ID NO:8
(i) sequence signature
(A) length: 41 bases
(B) type: nucleic acid
(C) chain: strand
(D) topological framework: linearity
(ii) molecule type: oligonucleotide (xi) sequence description: the information of SEQ ID NO:8:TGAACAGCGGCGGCGGCTTCGGTTTGGGCTTAGGCTTCGGC 41 (10) SEQ ID NO:9
(i) sequence signature
(A) length: 41 bases
(B) type: nucleic acid
(C) chain: strand
(D) topological framework: linearity
(ii) molecule type: oligonucleotide (xi) sequence description: SEQ ID NO:9:TGAACAGCGGCGGCGGCTTCAGTTTGGGCTTAGGCTTCGGC 41
Claims (18)
1, a kind of isolated polypeptide-human glutaminyl tRNA synthetic enzyme 23.76 is characterized in that it includes: the polypeptide of the aminoacid sequence shown in the SEQ IDNO:2 or the active fragments of its polypeptide, analogue or derivative.
2, polypeptide as claimed in claim 1, the aminoacid sequence that it is characterized in that described polypeptide, analogue or derivative has the homogeny with the aminoacid sequence at least 95% shown in the SEQ ID NO:2.
3, polypeptide as claimed in claim 2 is characterized in that it comprises the polypeptide with the aminoacid sequence shown in the SEQ ID NO:2.
4, a kind of isolating polynucleotide, it is characterized in that described polynucleotide comprise be selected from down the group in a kind of:
(a) coding have aminoacid sequence shown in the SEQ ID NO:2 polypeptide or its fragment, analogue, derive
The polynucleotide of thing;
(b) with polynucleotide (a) complementary polynucleotide; Or
(c) with (a) or the polynucleotide of at least 70% homogeny (b) are arranged.
5, polynucleotide as claimed in claim 4 is characterized in that described polynucleotide comprise coding and have SEQ
The polynucleotide of aminoacid sequence shown in the ID NO:2.
6, polynucleotide as claimed in claim 4, the sequence that it is characterized in that described polynucleotide include the sequence of 1-4070 position among the sequence of 83-733 position among the SEQ IDNO:1 or the SEQ ID NO:1.
7, a kind of recombinant vectors that contains exogenous polynucleotide is characterized in that it is the recombinant vectors that is formed by the described polynucleotide of arbitrary claim among the claim 4-6 and plasmid, virus or vehicle expression vector establishment.
8, a kind of genetically engineered host cell that contains exogenous polynucleotide is characterized in that it is to be selected from following a kind of host cell:
(a) host cell that transforms or transduce with the described recombinant vectors of claim 7; Or
(b) host cell that transforms or transduce with the described polynucleotide of the arbitrary claim among the claim 4-6.
9, a kind of preparation method with human glutaminyl tRNA synthetic enzyme 23.76 active polypeptide is characterized in that described method comprises:
(a) under expressing human glutamy tRNA synthetic enzyme 23.76 conditions, cultivate the described through engineering approaches host cell of claim 8;
(b) from culture, isolate and have human glutaminyl tRNA synthetic enzyme 23.76 active polypeptide.
10, a kind of can with polypeptide bonded antibody, it is characterized in that described antibody be can with human glutaminyl tRNA synthetic enzyme 23.76 specificity bonded antibody.
11, the compound of an analoglike or adjusting polypeptide active or expression is characterized in that they are simulation, promotion, antagonism or the active compound that suppresses human glutaminyl tRNA synthetic enzyme 23.76.
12, compound as claimed in claim 11 is characterized in that it is the polynucleotide sequence shown in the SEQ ID NO:1 or its segmental antisense sequences.
13, the described application of compound of a kind of claim 11, it is characterized in that described compound be used for mediator's glutamy tRNA synthetic enzyme 23.76 in vivo, the method for external activity.
14, a kind of disease relevant or method of disease susceptibility of detecting with the described polypeptide of arbitrary claim among the claim 1-3, it is characterized in that it comprises the described polypeptide expression amount that detects, perhaps detect the activity of described polypeptide, perhaps detect and cause described expression of polypeptides amount or active unusual nucleotide diversity in the polynucleotide.
15, as the application of polypeptide as described in the arbitrary claim among the claim 1-3, it is characterized in that it is applied to screen stand-in, the agonist of human glutaminyl tRNA synthetic enzyme 23.76, antagonist or inhibitor; Perhaps be used for the peptide finger print identification.
16, as the application of the described nucleic acid molecule of arbitrary claim among the claim 4-6, it is characterized in that it is used for nucleic acid amplification reaction as primer, perhaps be used for hybridization, perhaps be used to make gene chip or microarray as probe.
17,, it is characterized in that forming pharmaceutical composition with safe and effective dosage and pharmaceutically acceptable carrier as the relevant unusually disease of diagnosis or treatment and human glutaminyl tRNA synthetic enzyme 23.76 with described polypeptide, polynucleotide or its stand-in, agonist, antagonist or inhibitor as the described polypeptide of arbitrary claim, polynucleotide or application of compound in claim 1-6 and 11.
18, the described polypeptide of arbitrary claim, polynucleotide or the application of compound among the claim 1-6 and 11, it is characterized in that being used for the treatment of as malignant tumour with described polypeptide, polynucleotide or compound, hemopathy, the medicine of HIV infection and immunological disease and all kinds of inflammation.
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|---|---|---|---|
| CN 01105087 CN1363660A (en) | 2001-01-05 | 2001-01-05 | Polypeptide-human glutamyl transfer RNA synthetase 23.76 and polynucleotide for coding it |
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| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| CN 01105087 CN1363660A (en) | 2001-01-05 | 2001-01-05 | Polypeptide-human glutamyl transfer RNA synthetase 23.76 and polynucleotide for coding it |
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| Publication Number | Publication Date |
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| CN1363660A true CN1363660A (en) | 2002-08-14 |
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| Application Number | Title | Priority Date | Filing Date |
|---|---|---|---|
| CN 01105087 Pending CN1363660A (en) | 2001-01-05 | 2001-01-05 | Polypeptide-human glutamyl transfer RNA synthetase 23.76 and polynucleotide for coding it |
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2001
- 2001-01-05 CN CN 01105087 patent/CN1363660A/en active Pending
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