CN101993919A - In-situ hybridization detection kit for PD-ECGF genes and detection method and application thereof - Google Patents

In-situ hybridization detection kit for PD-ECGF genes and detection method and application thereof Download PDF

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CN101993919A
CN101993919A CN 200910056155 CN200910056155A CN101993919A CN 101993919 A CN101993919 A CN 101993919A CN 200910056155 CN200910056155 CN 200910056155 CN 200910056155 A CN200910056155 A CN 200910056155A CN 101993919 A CN101993919 A CN 101993919A
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hybridization
ecgf
cancer
marker
application
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裘建英
张云福
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Ruiqu Biotechnology Shanghai Co Ltd
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Ruiqu Biotechnology Shanghai Co Ltd
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Abstract

The invention relates to an in-situ hybridization detection kit for platelet derived endothelial cell growth factor (PD-ECGF) genes, which comprises a hybridization probe and a marker, wherein the sequence of the hybridization probe is expressed as SEQ ID No.1. The invention also provides an in-situ hybridization detection method for the PD-ECGF genes. In addition, the invention also provides application of the kit in preparation a medicament for detecting early cancer transfer and recurrent diseases. The kit provided by the invention has the advantages of high sensitivity and strong specificity. The detection method is convenient and easy to operate, and can be universally used and popularized in hospitals of above district level.

Description

A kind of hybridization in situ detection kit of PD-ECGF gene and detection method thereof and application
[technical field]
The present invention relates to a kind of test kit, specifically about a kind of hybridization in situ detection kit and detection method and application of PD-ECGF gene
[background technology]
An annual report has been done by how tame units such as U.S. sanitary research institute in 2005, cancer research institute, Disease Control and Prevention Center, " think that the mankind are failures in anticancer Great War ", that is to say that cancer mortality does not reduce, it lists and causes the Several Factors of anticancer Great War failure to be: 1, tumour cell heterogeneity; 2, tumor cell drug resistance; 3, cancer therapy drug mentality of designing imperfection etc.Simultaneously, also propose to examine closely again the measure of existing diagnosis and treatment cancer in this report.The inventor finds that under study for action two major reasons in addition that cause cancer mortality not fallen are: 1, can not accomplish real early diagnosis; 2, the pathomechanism of Zhuan Yiing is unclear.Come diagnosing cancer according to traditional medical image and with other biochemistry (as protein marker) index, think that occupancy cancer piece is the diagnosis (littler asymptomatic sometimes sign) that belongs to early-stage cancer under 2 centimeters, this clinical concept is worth conscientiously discussing.It is rigorous inadequately that 2 centimeters early stage these of following cancer pieces genus of medical imaging define science, from the cytology angle, 1 centimeter lump has 100,000,000 tumour cells approximately, its three-dimensional cell stack number of 2 centimeters lump is far above 200,000,000 tumour cells, produce and form 2 centimeters cancer piece to the mono-clonal cancer cells early stage from canceration, its pathology evolution process is quite long, may be more than 1 year or 2 years even 3 years, what be difficult to confirm is in this process, and lump is unique spot of cancer and independent focus.Confirm clinically: in case when forming lump, other cancer cells are moved to other position clonal growths by different approaches; In case behind the excision primary tumor, other organ recurrence kitchen ranges or multiple cancer piece kitchen range successively form or shift.Therefore, whether define in early days rigorous inadequately (some case clinically with the lump size below 2 centimeters, when finding primary lesion, find metastatic lesion simultaneously, not in the content of our statement), at this moment be late period, this is the true cause that causes cancer mortality not fallen.
Platelet-derived endothelial cell growth factor (ECGF) (platelet derived endothelial cell growth factor, PD-ECGF) from fresh blood platelet solute, extract the earliest, thereafter confirmation is with a kind of material with thymidine phosphorylase (TP), and its gene is positioned at chromosome 22 q13 ".PD-ECGF expression rate in liver cancer tissue reaches 67.8%~70.5%, is higher than cancer Zhou Zhengchang hepatic tissue, and organizes in the liver cancer to express at the TNM height by stages and be higher than the low group by stages of TNM; In the hepatocellular carcinoma with TTPV, the PD-ECGF expression level is higher than without the TTPV person, prompting PD-ECGF may with the associated angiogenesis in liver cancer growth and the Invasion and Metastasis, the PD-ECGF level can be used as the prediction index of hepatoma Metastasis recurrence.Usefulness immunohistochemical methods methods such as Volm have been studied the expression of PD-ECGF, bFGF and VEGF in the 168 routine non-small cell lung cancerous tissues, find in 3 equal negative patients of index that 43% has nodus lymphoideus transferring rate, and among 3 equal male patients of index 77% nodus lymphoideus transferring rate takes place, two groups exist significant difference.Confirmed all that in mRNA level, protein expression and enzyme activity assay PD-ECGF plays an important role in the malignant progression of tumours such as bladder cancer.PD-ECGFmRNA expresses high more, and the local infiltration scope is wide more, easy more lymphoglandula or the distant metastasis of occurring, and prognosis is poor more.
Along with molecular biotechnology is perfect day by day, functional genomics, the deep expansion of research such as cancer genomics, so far, we might do more accurate early diagnosis on gene level, just can accomplish the early prediction diagnosis in canceration early stage or cancer cells formation (during mono-clonal).Adopt nucleic acid hybridization in situ technology for detection PD-ECGF gene, the transfer diagnosis of the early gene level of cancer is had very important clinical meaning.PD-ECGF (platelet-derived endothelial cell growth factor (ECGF)) gene, gene order number: NM_001014440,970bp, mRNA.22q13.33 ", CDS:138 ... 899bp.
Hybridization in situ technique (in situ hybridization) combines molecular biology and cytochemistry technology, is probe with the nucleic acid molecule of mark, in the technology of histocyte in situ detection specific nucleic acid molecule.Its principle is to make the nucleic acid strand (being probe) that contains distinguished sequence, process mark, under optimum conditions with histocyte in the complementary nucleic acid strand be that target nucleic acid is hybridized, with radioautograph or immunocytochemistry label probe is surveyed again, thereby shown special DNA or RNA molecule at cell in-situ.
[summary of the invention]
The objective of the invention is provides a kind of purposes of hybridization in situ detection kit of PD-ECGF gene at deficiency of the prior art.
One purpose more of the present invention is that a kind of hybridization in situ detection kit of PD-ECGF gene is provided.
Another purpose of the present invention is that a kind of in situ hybridization detection method of PD-ECGF gene is provided.
For achieving the above object, the technical scheme taked of the present invention is:
A kind of hybridization in situ detection kit of PD-ECGF gene detects cancer in preparation and shifts, recurs application in the disease medicament in early days, and described test kit comprises hybridization probe, marker, and described hybridization probe sequence is shown in SEQ ID NO.1.
Described cancer is liver cancer or bladder cancer.
The RNA sequence of described hybridization probe sequence shown in SEQ ID NO.1.
Described marker is selected from radionuclide or non-radioactive marker.
Described radionuclide is selected from 3H, 35S, 125I or 32A kind of among the P.
Described non-radioactive marker is selected from a kind of in vitamin H, digoxin, alkaline phosphatase, horseradish peroxidase or the fluorescein.
Described non-radioactive marker is preferably from digoxin.
Described test kit also comprises synergistic agent, and described synergistic agent is the alkaline phosphatase enzyme antibody.
For realizing above-mentioned second purpose, the technical scheme that the present invention takes is:
A kind of hybridization in situ detection kit of PD-ECGF gene comprises hybridization probe, marker, and wherein said hybridization probe sequence is shown in SEQ ID NO.1, and described marker is selected from radionuclide or non-radioactive marker.
For realizing above-mentioned the 3rd purpose, the technical scheme that the present invention takes is:
A kind of in situ hybridization detection method of PD-ECGF gene, this method may further comprise the steps:
A, the hybridization probe in the test kit is contacted with RNA to be measured in the substrate, form hybridization complex;
The hybridization complex that b, detection a step obtain.
The component of diagnostic kit of the present invention is by hybridization probe, hybridization solution, developer, compositions such as synergistic agent.The nucleic acid hybridization principle of this test kit is that the molecular biology insider all knows, and the concrete operations step is to carry out quantitative analysis, result's report under sample disposal, prehybridization, hybridization, immunohistochemical staining, the mirror, and wherein Za Jiao concrete steps comprise:
Instrumentation:
1). sample to be measured is put into reactive tank;
2). instrument discards liquid automatically, adds Digestive system automatically;
3). instrument discards liquid automatically, and the back is fixing automatically;
4). instrument discards liquid automatically, automatically prehybridization (42 ℃);
5). instrument discards liquid automatically, cleans automatically;
6). instrument discards liquid automatically, automatically hybridization (42 ℃);
7). instrument discards liquid automatically, cleans automatically;
8). instrument discards liquid automatically, and automatic and DIG antibody is cultivated (room temperature);
9). instrument discards liquid automatically, cleans colour developing automatically;
10). take out the mounting microscopy.
The invention has the advantages that:
1, test kit provided by the invention has characteristics highly sensitive, high specificity.
2, detection method of the present invention is convenient and simple for operation, can be widely used and promoted in Municipal Hospitals.
3, diagnostic kit of the present invention and other detection oncofetal protein mark clinically, and the medical imaging inspection has remarkable difference.The present invention can detect the PD-ECGF gene unconventionality expression on gene level, before the recurrence of occupancy carninomatosis kitchen range is not found in the medical imaging inspection, before the cancer biochemical indicator does not produce unusually, also do not form before the tumour, can accomplish the information acquisition of above abnormal gene expression early, predict for real early diagnosis of clinical cancer sufferer and treatment back transfer and relapse early.So just might implement early diagnosis, early prevention, the early treatment of cancer, might from the source, thoroughly effect a radical cure the cancer foul disease.
[description of drawings]
Fig. 1 is a hepatoma Metastasis patient P D-ECGF genetic expression picture in the embodiment of the invention.
Fig. 2 is that bladder cancer shifts patient P D-ECGF genetic expression picture in the embodiment of the invention.
Fig. 3 is a normal people PD-ECGF genetic expression picture in the embodiment of the invention.
[embodiment]
Below in conjunction with accompanying drawing the specific embodiment of the invention is elaborated.
Embodiment 1
A kind of hybridization in situ detection kit of PD-ECGF gene comprises hybridization probe, marker, synergistic agent, and wherein, described hybridization probe sequence is shown in SEQ ID NO.1.The hybridization probe digoxigenin labeled.Other liquid and sample in the test kit are composed as follows:
Digestive system 100 μ l/ manage 1 pipe/box colourless transparent liquid
Protection liquid 100 μ l/ pipe 1 pipe/box colourless transparent liquid
Prehybridization solution 1300 μ l/ manage 2 pipe/box colourless transparent liquids
Justice hybridization solution 10 μ l/ pipe 1 pipe/box colourless transparent liquid
Antisense hybridization solution 10 μ l/ manage 1 pipe/box colourless transparent liquid
Confining liquid 1000 μ l/ manage 1 pipe/box colourless transparent liquid
Alkaline phosphatase enzyme antibody 1 μ l/ manages 1 pipe/box colourless transparent liquid
Developer A 175 μ l/ manage 1 pipe/box yellow liquid
Developer B 320 μ l/ manage 1 pipe/box colourless transparent liquid
Light yellow or the colourless transparent liquid of damping fluid I 10x 90ml/ bottle 1 bottle/box
Light yellow or the colourless transparent liquid of damping fluid II 10x 80ml/ bottle 1 bottle/box
Light yellow or the colourless transparent liquid of damping fluid III 10x 20m/ bottle 3 bottle/boxes
Light yellow or the colourless transparent liquid of damping fluid IV 10x 90ml/ bottle 1 bottle/box
Stationary liquid 90ml/ bottle 1 bottle/box colourless transparent liquid
6/box of positive control sample
Mentioned reagent composition explanation: (all reagent are available from SIGMA)
1, Digestive system: the 20mg/ml Proteinase K, the 100mg Proteinase K adds DEPC-H 2O 5ml;
2, the glycine of protection liquid: 0.2g adds 1 * damping fluid I of 1ml;
3, prehybridization solution: 1 * damping fluid II 7.5ml
50×D?3ml
10mg/ml?yest?t-RNA?750ul
11mg/ml?SALMON?TESTES?DNA 682ul
0.04M?EDTA?3ml
50%formamide?15ml
4, the bloking of confining liquid: 0.03g (buying from Roche Holding Ag) adds 1ml 1 * damping fluid III;
5,10x damping fluid I:(PH7.1-7.4)
NaCl?80g
Na 2HPO 4.12H 2O 360g
KCl 2g
KH 2PO 42g
Add tri-distilled water to 1l, and autoclaving;
6,10x damping fluid II:(PH7.0)
NaCl 175.3g
Trisodium Citrate 88.2g
Several of HCl
Add tri-distilled water to 1l, and autoclaving;
7, damping fluid III:(PH7.9)
Tris 121.1g
NaCl?87.66g
About HCl 60ml
Add tri-distilled water to 1l, and autoclaving;
8, damping fluid IV:
1M Tris-HCl (PH9.5): Tirs 121.1g adds about HCl 3ml, adds water 900ml, transfers PH to 9.5, adds water to 1l, and autoclaving;
1M NaCl:NaCl 58.44 adds water to 1l, and autoclaving;
0.5M MgCl 2: 101.65g MgCl 2.6H 2O adds water to 1l, and autoclaving;
9, stationary liquid: Paraformaldehyde 96 40g adds 1 * damping fluid I to 1l, and heat (about 50-60 degree) is stirred to dissolving a little;
10, developer A:NBT 1g adds 70%DMF11.44ml;
11, developer B:BCIP 1g adds 100%DMF30ml.
Test kit of the present invention can many person-portions use or person-portion use.
Embodiment 2
A kind of PD-ECGF gene hybridization in situ detection method and test kit thereof are used
One, sample disposal
1, with the centrifuge tube of 10ml, dress 4.5ml lymphocyte separation medium, again the 3ml anticoagulation is slowly added contain lymphocyte separation medium (blood: in centrifuge tube lymphocyte separation medium=1: 1.5), the centrifugal 10min of 2000r/min;
2, draw the middle layer white corpuscle to another centrifuge tube, in this pipe, add 1 * damping fluid I of about twice again, mixing, the centrifugal 10min of 1500g/min;
3, abandon supernatant. precipitation adds 1 * damping fluid I of about twice, mixing, the centrifugal 10min of 1500g/min;
4, abandon supernatant, and test tube mouth excess liquid is gone with the tissue suction.Again precipitation is made suspension, drop in push jack on the slide, seasoning.(hospital with good conditionsi can use the pelleter film-making.) 3ml blood, can do 4 slice, thin pieces;
5, with 40ml 4% stationary liquid, in glass jar, fixedly 30min uses 1 * damping fluid I to wash 5min again.Every cylinder can be put 16;
6, sample can be kept at-20 ℃, or continues to do experiment.
Two, reagent in the test kit is mixed with working concentration
1, with 10 * damping fluid I with tri-distilled water by being diluted to 1 * damping fluid I at 1: 10;
2, with 20 * damping fluid II with tri-distilled water by being diluted to 2 * damping fluid II at 1: 10;
By being diluted to 0.2 * damping fluid II at 1: 100; By being diluted to 0.1 * damping fluid II at 1: 200;
3, with 10 * damping fluid III with tri-distilled water by being diluted to 1 * damping fluid III at 1: 10;
4,10 * damping fluid IV with tri-distilled water by be diluted at 1: 10 * damping fluid IV (get 1#, 2#, each 10ml of 3#, add water to 100ml both can).
Three, experimental procedure:
1, gets two of every person's samples to be checked, two of (other two give over to check with) and positive control samples (test at every turn and do a pair of positive control);
2, in glass jar, add Digestive system (Digestive system 100ul adds 1 * damping fluid 199.9ml, is working concentration) 20ml.37 ℃ of water-bath preheatings 10 minutes.Put 16 slides into, handle 12min, use 1 * damping fluid I to wash 5min again for 37 ℃;
3, wash 10min with 0.2% protection liquid (protection liquid 1ml adds 1 * damping fluid I99ml and is working concentration), tri-distilled water is washed 5min, and above process is all carried out at glass jar.The slide seasoning;
4, slide is put into the box of preserving moisture, add prehybridization solution 20ul/ sheet. covered, the lid box of tightly preserving moisture is placed in 42 ℃ of constant water bath box more than the 3h;
5, take out slide, discard cover glass, slide is put into glass jar, with 70%, 90%, 95% ethanol is respectively washed 2min, seasoning;
6, slide is put into the box of preserving moisture, two of every patient specimens, one adds just hybridization solution 20ul/ sheet, and another adds antisense hybridization solution 20ul/ sheet, covered, the lid box of tightly preserving moisture is placed on 16-24h in 42 ℃ of constant water bath box;
7, take out slide, discard cover glass, slide is put into glass jar
In 42 ℃ of constant water bath box, wash twice, each 15min with 2 * damping fluid II
In 42 ℃ of constant water bath box, wash once each 15min with 0.2 * damping fluid II
In 42 ℃ of constant water bath box, wash twice, each 15min with 0.1 * damping fluid II;
8, wash 30s with 1 * damping fluid III, take out slide, seasoning;
9, slide is put into the box of preserving moisture, add 0.5%l confining liquid (the 1ml confining liquid adds 5ml1 * damping fluid III) 100ul/ sheet, cover the box of tightly preserving moisture, at room temperature act on 30min;
10, take out slide, III washes 30s with 1 * damping fluid, seasoning;
11, slide is put into the box of preserving moisture, add alkaline phosphatase enzyme antibody (adding 1.8ml 1 * damping fluid III) 100ul/ sheet, cover the box of tightly preserving moisture and at room temperature act on 30min;
12, take out slide, wash 3 times, each 15min with 1 * damping fluid III;
13,1 * damping fluid IV washes 2min, adds developer (developer A73.3ul, developer B157.5ul are added among 30ml 1 * damping fluid IV, mixing), more than the room temperature lucifuge 12h;
14, wash 5min with tri-distilled water, seasoning, (add with glycerine 10% 1 * damping fluid I mixing) mounting microscopy.
Four, the result judges
100-300 cell of counting calculates the per-cent of catching the purple cell under light microscopic.
What the positive control sample added the antisense hybridization solution should catch purple more than 80%.
All add the negative internal reference of just hybridization solution should be colourless.
The cDNA of digoxigenin labeled, RNA and oligonucleotide probe, not only probe has a biotin labeling advantage, also having overcome biotin labeled probe is organized the endogenous vitamin H to do shortcomings such as sorrow in the crossover process in position), this hybridization probe and the leukocytic RNA nucleic acid to be measured of blood of human body are hybridized, method with immunohistochemical methods develops the color again, under light microscopic, observe existence and the location of mRNA,, judge the expression amount of goal gene according to painted cell count.
The inventive method is a nucleic acid hybridization in situ technology at present commonly used, and this method is by detecting the PD-ECGF gene expression amount in the substrate cell, is used for determining whether cancer takes place and/or shift.
Clinical study shows that the PD-ECGF gene has broad spectrum, because the PD-ECGF gene is expressed low in the normal people or zero expression.If the PD-ECGF gene high expression illustrates that cancer recurs, shifts, spreads, thus the diagnostic message of the gene level of acquisition cancer.When detecting the PD-ECGF expression of gene and be higher than normal control, to be that cancer is early stage shift or the cancer metastasis susceptible person then measurable experimenter, and these cancers comprise liver cancer or bladder cancer.
The embodiment of the invention is sampled as: 5 of hepatoma Metastasis patients, bladder cancer shifts 5 of patients, 5 of normal control groups.Take out all people's to be checked peripheral blood 3-5 milliliter (separation white corpuscle) and do in situ hybridization.The result represents that all cancer metastasis patient P D-ECGF genes have overexpression, cell dyeing; Normal control group PD-ECGF gene is not expressed the cell dye-free.Concrete outcome is asked for an interview Fig. 1, Fig. 2 and Fig. 3.
Embodiment 3
Detecting bladder cancer with the PD-ECGF kit gene shifts disease and detects parallel laboratory test between the bladder cancer transfer disease with the CA125 kit gene.
Shift specificity, susceptibility, the accuracy of disease for each comfortable bladder cancer of scientific evaluation said gene.We use the method for parallel test, detect the mRNA of said gene simultaneously, detection technique adopts the nucleic acid hybridization in situ technology, shift the disease peripheral blood of patients with same routine bladder cancer, detect PD-ECGF gene and CA125 gene simultaneously, NM-024690, (carrying out same procedure and step and reagent that the hybridization in situ technique of embodiment 1 and embodiment 2 is all adopted in nucleic acid hybridization in situ, immunohistochemical staining, mirror numeration down, report as a result etc.).Find that the PD-ECGF gene shifts among the disease patient expression amount than the expression amount height of CA125 gene same disease patient in bladder cancer.The result shows that it is better than CA125 gene that PD-ECGF gene pairs bladder cancer shifts specificity, susceptibility, the accuracy of medical diagnosis on disease, and in situ hybridization genetic expression figure shows that PD-ECGF expression of gene amount is 70%, and CA125 expression of gene amount is 47%.The index that test kit of the present invention is done in transfer medicals diagnosis on disease such as bladder cancer has very important clinical meaning.
SEQUENCE?LISTING
<110〉Rui bends biotechnology (Shanghai) Co., Ltd.
<120〉a kind of hybridization in situ detection kit of PD-ECGF gene and detection method thereof and application
<130>/
<160>1
<170>PatentIn?version?3.3
<210>1
<211>970
<212>DNA
<213〉homo sapiens (Homo sapiens)
<400>1
gaagcgggaa?agggccacaa?tggggtctgg?gaggtgggcg?gggcggagcg?gggatgtcca 60
gccacgtcgc?tttgttttcc?cacgctagga?gctaccacaa?caggtgctgc?gagccgtaag 120
cgccccccac?ccgcgctatg?ggctcggacg?cctgggtggg?cctttggcgg?ccacaccggc 180
cccgcggccc?catcgcggcg?cactacggag?gccccgggcc?caaatacaag?ctgccgccca 240
acaccggcta?cgccctgcat?gacccgtcgc?ggccgcgcgc?ccccgccttc?accttcggcg 300
cgcgcttccc?cacgcagcag?acgacgtgcg?gccccgggcc?aggccacctg?gtgcccgctc 360
gcatgaccgt?gcgcggcacc?gacggcgccc?ccgcctactc?catctacggc?cgcccacgcc 420
gctcagcgcc?cttcctcact?ccgggacctg?gcaggtactt?cccggagcga?gcggggaacg 480
cgacgtaccc?cagtgcgcct?cggcacacca?ttgctccccg?aaactggggt?gtccaggcgg 540
aacagcagag?cccaggtccc?gcggcctata?cggtgccctc?gctcttgggt?ccgcgcgtca 600
tcggcaaagt?ctccgcccca?acttgctcca?tctacggccg?cagagcggct?ggcagtttct 660
tcgaggacct?cagcaagacc?ccgggcccct?gcgcctatca?ggtcgtgagt?ccaggggtct 720
acaagtcccg?ggccccccag?ttcacgattc?tggcgcggac?ttcgctcccc?caagacaaca 780
ctcggaagcc?agggcccgcg?gcctacaacg?tggatcagca?ccggaagccc?cgcggctgga 840
gtttcgggat?ccggcactcg?gactacctgg?ccccgctggt?gaccgacgcg?gacaactgac 900
ccgccaggcg?ggagcggccc?cacacgtgtt?tgcttaaagt?ctgcgagtcc?gcatcgtgtc 960
cgcctctctc 970

Claims (11)

1. the hybridization in situ detection kit of a PD-ECGF gene detects cancer in preparation and shifts, recurs application in the disease medicament in early days, and described test kit comprises hybridization probe, marker, and described hybridization probe sequence is shown in SEQ ID NO.1.
2. application according to claim 1 is characterized in that: described cancer is liver cancer or bladder cancer.
3. application according to claim 1 is characterized in that: the RNA sequence of described hybridization probe sequence shown in SEQ ID NO.1.
4. according to the arbitrary described application of claim 1-3, it is characterized in that: described marker is selected from radionuclide or non-radioactive marker.
5. application according to claim 4 is characterized in that: described radionuclide is selected from 3H, 35S, 125I or 32A kind of among the P.
6. application according to claim 4 is characterized in that: described non-radioactive marker is selected from a kind of in vitamin H, digoxin, alkaline phosphatase, horseradish peroxidase or the fluorescein.
7. application according to claim 6 is characterized in that: described non-radioactive marker is preferably from digoxin.
8. according to the arbitrary described application of claim 1-3, it is characterized in that: described test kit also comprises synergistic agent, and described synergistic agent is the alkaline phosphatase enzyme antibody.
9. the hybridization in situ detection kit of a PD-ECGF gene comprises hybridization probe, marker, it is characterized in that, described hybridization probe sequence is shown in SEQ ID NO.1, and described marker is selected from radionuclide or non-radioactive marker.
10. the in situ hybridization detection method of a PD-ECGF gene is characterized in that, this method may further comprise the steps:
A, the hybridization probe in the described test kit of claim 9 is contacted with RNA to be measured in the substrate, form hybridization complex;
The hybridization complex that b, detection a step obtain.
11. detection method according to claim 10 is characterized in that: the condition that forms hybridization complex in a step is: the temperature of nucleic acid hybridization is 42 ℃; The time of nucleic acid hybridization is 16-24 hour, and described substrate is selected blood cell sample or histocyte sample for use.
CN 200910056155 2009-08-10 2009-08-10 In-situ hybridization detection kit for PD-ECGF genes and detection method and application thereof Pending CN101993919A (en)

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Cited By (1)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
CN107667292A (en) * 2015-03-11 2018-02-06 生物医学研究所(Idibell) Cancer markers PD ECGF

Cited By (6)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
CN107667292A (en) * 2015-03-11 2018-02-06 生物医学研究所(Idibell) Cancer markers PD ECGF
JP2018512585A (en) * 2015-03-11 2018-05-17 フンダシオ インスティトゥト ディンベスティガシオ ビオメディカ デ ベイビジャ(イ デ イ ベ エ エレ エレ)Fundacio Institut D‘Investigacio Biomedica De Bellvitge(Idibell) PD-ECGF as a biomarker for cancer
CN107667292B (en) * 2015-03-11 2020-06-19 生物医学研究所(Idibell) Cancer marker PD-ECGF
JP2020201278A (en) * 2015-03-11 2020-12-17 フンダシオ インスティトゥト ディンベスティガシオ ビオメディカ デ ベイビジャ(イ デ イ ベ エ エレ エレ)Fundacio Institut D‘Investigacio Biomedica De Bellvitge(Idibell) Pd-ecgf as biomarker of cancer
US11802874B2 (en) 2015-03-11 2023-10-31 Fundacio Institut D'investigació Biomèdica De Bellvitge (Idibell) PD-ECGF as biomarker of cancer
JP7453284B2 (en) 2015-03-11 2024-03-19 フンダシオ インスティトゥト ディンベスティガシオ ビオメディカ デ ベイビジャ(イ デ イ ベ エ エレ エレ) PD-ECGF as a cancer biomarker

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Application publication date: 20110330