CN108642184A - Application, kit and the detection method of kidney prognosis novel molecular marker non-coding RNA LINC00200 - Google Patents
Application, kit and the detection method of kidney prognosis novel molecular marker non-coding RNA LINC00200 Download PDFInfo
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Abstract
The present invention relates to a kind of application, kit and the detection methods of kidney prognosis novel molecular marker non-coding RNA LINC00200, it is related with the survival rate of patient by real-time fluorescence quantitative PCR and the survivorship curve analysis non-coding RNA LINC00200 for finding renal carcinoma tissue source, content is higher, survival rate is higher, this method provides strong technical support to predict that the prognosis life cycle of patients with renal cell carcinoma is analyzed, help to improve the postoperative life quality of patients with renal cell carcinoma, work out aftertreatment scheme, survival rate is improved, there is far-reaching clinical meaning.
Description
Technical field
The invention belongs to oncomolecularbiology fields, and in particular to a kind of kidney prognosis novel molecular marker non-coding
Application, kit and the detection method of RNA LINC00200.
Background technology
Kidney is the malignant tumour originating from kidney essence uriniferous tubule epithelial systems, and full name is clear-cell carcinoma, abbreviation kidney
Cancer.Include all kinds of different subtypes renal cell carcinomas originating from renal tubule different parts in histopathology, but does not include deriving from renal interstitial
Tumour and tumor of renal pelvis and urothelial tumor.Worldwide kidney incidence is not quite similar, and developed country is sent out on the whole
Sick rate is slightly above developing country, and men and women's patient morbidity's ratio is about 2:1, Gao Fa Nian Ling section is 50 years old or so.The world at present
Kidney incidence though radical operation can cure most of early stage patient, but still has nearly 30% in ascendant trend year by year in range
There is Local advancement and DISTANT METASTASES IN in patient, this some patients can not row radical operation for late period when medical.Currently, facing
On bed not yet ideal molecular indexes come the risk assessing prognosis and shift.Therefore, new prognosis biological marker is found
Object is current urgent problem.
The Human Genome Project, which discloses in human genome, 3,000,000,000 base-pairs, wherein only about 2% enough coding proteins.
Remaining 98% is non-protein encoding genes, these gene orders were considered as once " rubbish " or " voice ".Then research
It was found that about 75% human genome can be transcribed into RNA, wherein most is non-protein coding RNA.With genomics
With the fast development of bioinformatics, scientist is found that the transcript (i.e. non-coding RNA) of more and more non-protein codings,
Wherein long-chain non-coding RNA is proved to play a significant role with a variety of different mechanisms in numerous important biological processes.In life
In terms of reason, long-chain non-coding RNA participates in mammalian development process by regulating and controlling several genes expression;In terms of disease, long-chain
Non-coding RNA unconventionality expression occurs with tumour and the processes such as transfer are closely related.LINC00200 is a kind of newfound non-coding
RNA, transcript length are more than 200 nucleotide.Currently, LINC00200 is in normal cell development or tumor development
The important function played in the process is also in further research.Whether LINC00200 can be as a kind of new tumor markers
For predicting that prognosis of patients with renal cell carcinoma not yet has been reported that.Therefore, we are illustrated for the first time with LINC00200 as new kidney marker
To predict the feasibility of patient's prognosis.
Invention content
The object of the present invention is to provide a kind of answering for kidney prognosis novel molecular marker non-coding RNA LINC00200
With, secondly, the present invention provide a kind of detection marker non-coding RNA LIFR-AS in renal carcinoma tissue the kit of expression quantity and
Detection method.
The object of the present invention is achieved like this:
Kidney prognosis novel molecular marker non-coding RNA LINC00200 is preparing answering for the preparation of prediction prognosis of patients with renal cell carcinoma
With the nucleic acid sequence such as SEQ NO of non-coding RNA LINC00200:Shown in 1.
The preparation for predicting prognosis of patients with renal cell carcinoma is real-time fluorescence quantitative PCR detection kit.
Kit includes the specific primer for detecting non-coding RNA LINC00200 expression, the specific primer
Nucleic acid sequence be SEQ NO:2 and SEQ NO:The primer sequence that 3 and reference gene TUBA1A is expressed, the core of the primer
Acid sequence is SEQ NO:4 and SEQ NO:5.
Kit also contains all reagents for extracting RNA from tissue and carrying out reverse transcription and real-time fluorescence quantitative PCR, packet
Include (1) extracted total RNA agents useful for same from the tumour of kidney or normal control tissue, including Trizol liquid, chloroform, isopropanol,
Inhibit RNA degradations solvent, 75% ethyl alcohol, DEPC water;(2) it is by non-coding RNA LINC00200 reverse transcriptions by template of total serum IgE
CDNA agents useful for same, including reverse transcription reaction buffer solution, contain triphosphoric acid base deoxynucleotide dNTP, reverse transcription containing Mg2+
The mixture of enzyme M-MLV and random primer and Oligo dT primers;(3) by cDNA real-time fluorescence quantitative PCR agents useful for same, packet
Include LINC00200 real-time fluorescence quantitative PCRs specific primer, TUBA1A internal references Specific PCR primers, real time fluorescent quantitative SYBR
Dyestuff, the water without RNA enzyme.
The detection method of kidney prognosis novel molecular marker non-coding RNA LINC00200, includes the following steps:1)It receives
Collect kidney to be measured or normal control tissue;
2) extracting of RNA in organizing;
3)The reverse transcription of LINC00200 RNA, using cell total rna as template, reverse transcription obtains cDNA;
4)Using cDNA as template, real-time fluorescence quantitative PCR expansion is carried out using the specific primer of non-coding RNA LINC00200
Increase, detects non-coding RNA LINC00200 expression quantity.
Step 3)Middle reverse transcription reaction system is 5 × RT Buffer(Containing Mg2+ and dNTP)4 μ l, 10 × RT Primer
Mix(Oligo dT Primer and Random Hexamers mixtures)2 μ l, BeyoRT II M-MLV reverse transcriptases
(RNase H-)(Inhibitor containing RNase)2 μ l, DEPC-treated water, 2 μ l remove the Total RNA after gDNA
10μl。
Step 4)The expression quantity relative quantitation method of middle detection marker non-coding RNA LINC00200.
The beneficial effects of the invention are as follows:Renal carcinoma tissue source is found by real-time fluorescence quantitative PCR and survivorship curve analysis
Non-coding RNA LINC00200 it is related to the survival rate of patient, content is higher, and survival rate is higher, this method be prediction kidney suffer from
The prognosis life cycle analysis of person provides strong technical support, helps to improve the postoperative life quality of patients with renal cell carcinoma, makes
Aftertreatment scheme is ordered, survival rate is improved, there is far-reaching clinical meaning.
Description of the drawings
Fig. 1 is that real-time fluorescence quantitative PCR analyzes differential expressions of the LINC00200 in normal structure and kidney;
Prognosis of the non-coding RNA LINC00200 expression height in the tracing analysis renal carcinoma tissue sources for survival Fig. 2 to patients with renal cell carcinoma
It influences.
Specific implementation mode
The present invention is made the following instructions with reference to embodiment:
Embodiment 1:Kidney prognosis novel molecular marker non-coding RNA LINC00200 is preparing prediction prognosis of patients with renal cell carcinoma
Preparation application, marker non-coding RNA LINC00200 is used to prepare to the preparation of kidney prognosis, predicts patients with renal cell carcinoma
Situation.
Embodiment 2:The reagent for preparing detection non-coding RNA LINC00200 expression quantity is used to prepare prognosis of patients with renal cell carcinoma
Kit (being used for 30 secondary responses) 1. Trizo l20ml
2. inhibiting RNA degradation solvents 40ml;
3. chloroform 80ml;
4. isopropanol 80ml;
5. DEPC water 10ml;
6. the 100 μ l of mixture of 10 × random primer and Oligo dT primers;
7. 5 × reverse transcription reaction buffer solution, 150 μ l;
8. triphosphoric acid base deoxynucleotide dNTP 100 μ ls of the 10mM containing Mg2+;
9. 50 μ l of 200U/ μ l M-MLV reverse transcriptases;
10. SYBR Green qPCR Mix 500μl;
11. 3 μM of target gene LINC00200 specific primers(Its sequence such as SEQ NO:2 and SEQ NO:Shown in 3) 50μl;
12. 3 μM of reference gene TUBA1A specific primers(Its sequence such as SEQ NO:4 and SEQ NO:Shown in 5) 50μl.
Embodiment 3:The detection of tissue samples non-coding RNA LINC00200
1, kidney to be measured or normal control tissue are collected, after physiological saline cleans up, is put into and fills inhibition RNA degradation solvents
In cryopreservation tube, put spare to -80 DEG C of refrigerators.
2, the extracting of RNA in organizing:
(1)Liquid nitrogen is first added in mortar, then tissue is cut into small pieces and is clayed into power in liquid nitrogen, is taken with the spoon of Liquid nitrogen precooler
100mg organizes powder to be added in the EP pipes for the Trizol liquid for having filled 1ml, and tissue total powder volume is no more than Trizol used
The 10% of volume is sufficiently mixed uniformly;
(2)5 minutes are placed at room temperature for, the chloroform of 200 μ l is then added, EP is covered tightly and manages and acutely sway 0.5 minute, 12000 revs/min
Zhongli's heart 10 minutes;
(3)Take upper strata aqueous phase in a new EP pipes(The intermediate beds of precipitation and subnatant are not mixed into), 500 μ l isopropanols are added,
Mildly reverse mixing, is placed at room temperature for 10 minutes, and 12000 revs/min centrifuge 10 minutes.
(4)Liquid is carefully discarded supernatant, is added 75% ethyl alcohol of 1ml, vortex mixing, 12000 revs/min of centrifugations 5 at 4 DEG C
Minute, repetitive operation is primary;
(5)Discard supernatant liquid(Residual liquid is removed as possible), room temperature or vacuum drying 5~10 minutes(It is careful not to dried
Point, it otherwise can reduce the solubility of RNA), RNA is dissolved with 50 μ l DEPC processed water;
(6)RNA concentration mensurations:It is measured with nucleic acid concentration analyzer, inhales 1 μ l RNA samples and add to sample well, according to reading
Directly determine the concentration of RNA;The OD260/OD280 ratios of the measurement of nucleic acid concentration analyzer, ratio are thought between 1.8-2.0
RNA purity is fine, and finally, it is spare that RNA is stored in -80 DEG C of refrigerators.
3, the reverse transcription of LINC00200 RNA:Use the Reverse Transcriptase kit of the green skies Bioisystech Co., Ltd in Shanghai
(D7170S), it is as follows:
(1)Remove genomic DNA:Template Total RNA, 5 × gDNA Eraser Buffer are thawed on ice, 5 × RT
Buffer, 10 × RT Primer Mix, DEPC-treated Water are immediately placed in (15-25 DEG C) defrosting of room temperature after defrosting
On ice, using preceding by each solution mixing and it is of short duration centrifugation so that all liq is settled down to tube bottom, the denaturation of RNA, RNA samples
Product thermal denaturation under the conditions of 65 DEG C is immediately placed on cooling in ice water, according to the form below ingredient is in the mixing of preparation reaction on ice after 5 minutes
Then liquid is dispensed into each reaction tube, is eventually adding RNA sample again;
(2)In PCR instrument or in water-bath, 37 DEG C be incubated 2 minutes, be immediately placed in place on ice it is spare;(3)Reverse transcription system is matched
System:Reaction solution preparation is carried out on ice, reverse transcription reaction is carried out immediately after soft mixing, according to the reverse transcription reaction system of following table
Prepare mixed liquor;
(4)42 DEG C are incubated 60 minutes to carry out reverse transcription reaction, and subsequent 80 DEG C of incubations are put in for 10 minutes after inactivation reverse transcriptase
On ice, for the template of secondary structure complexity or high GC content, reverse transcription temperature can be improved to 50 DEG C, to enhance reverse transcription effect
Rate;(5)Obtained cDNA can immediately or -80 DEG C freeze after be used for follow-up real-time fluorescence quantitative PCR, cDNA preferably avoids excessive
Multigelation.
4, real-time fluorescence quantitative PCR is carried out using the specific primer of non-coding RNA LINC00200:Specific primer exists
Raw work bioengineering(Shanghai)Limited liability company synthesizes, and includes for detecting the special of non-coding RNA LINC00200 expression
Property primer, primer sequence be SEQ NO:2 and SEQ NO:The primer sequence that 3 and reference gene TUBA1A is expressed, primer sequence
For SEQ NO:4 and SEQ NO:5, the other reagents of real-time fluorescence quantitative PCR utilize the green skies Bioisystech Co., Ltd in Shanghai
BeyoFast SYBR Green qPCR Mix (2 ×), are as follows:
(1)Melt and mixing PCR reacts required various solution, BeyoFast SYBR Green qPCR Mix melt completely
And mixing is placed in ice chest;(2)PCR reaction systems (by taking 96 orifice plates as an example) are set on ice bath:
(3) the usually amount of DNA profiling with 1-10ng cDNA is with reference to dosage, and final concentration of 0.2-0.5 μM of primer when can be obtained
Good detection result is obtained, the final concentration of primer also can be according to circumstances adjusted;If it is necessary, gradient dilution can be carried out to template,
With the template usage amount that determination is best;When reverse transcription PCR cDNA obtained by the reaction is directly as template, additive amount does not exceed
PCR reacts the 10% of total volume, and the recommendation response system of 96 orifice plates is 20 μ l, can also in proportion be expanded according to actual experiment demand
Big or diminution reaction system;
(4) mixing or slight Vortex mixings are gently blown and beaten with pipettor, room temperature centrifuges the several seconds, liquid is made to accumulate in tube bottom;
(5) the PCR reaction tubes set or PCR reaction plates are placed on fluorescence quantitative PCR instrument, start PCR reactions;(6) PCR reacts
Program:The pre-degeneration that template is carried out before real-time fluorescence quantitative PCR reacts, is typically set at 95 DEG C 2 minutes, using following
PCR programs, this program are by taking ABI 7900HT fluorescence quantitative PCR instruments as an example:A. pre-degeneration:95℃ 2min ;B. it is denaturalized:
95℃ 15sec;C. annealing/extension:60℃ 15-30sec;D. step b and step c is repeated, in total 40 cycles; e.
Melting curve analysis (optional):95℃ 15sec, 60℃ 15sec, 95℃ 15sec;F. it is carried using fluorescence quantitative PCR instrument
The software analysis result of confession;Three-step approach need to only add 72 DEG C of 30sec of a step after annealing/extension, then repeat step b, c and increasing
Add the step for totally 40 cycle.
5, the data analysis of non-coding RNA LINC00200 expression quantity:This experimental data be included in 60 patients with renal cell carcinoma and its
Normal control tissue.The interpretation of result of real-time quantitative PCR uses relative quantitation method, that is, 2^- △ △ Ct methods.It is specific as follows:It is first
First, all gene C t values once tested are put in order, later with the target gene LINC00200's in each group of tumor sample
Ct values subtract the Ct values of itself reference gene TUBA1A, and obtained number is exactly △ Ct;Changing formula into is exactly:△Ct=Ct(Purpose base
Because of LINC00200)-Ct(Reference gene TUBA1A);Then, by each group of each target gene of tumor sample LINC00200
△ Ct all calculate.The △ Ct of normal control tissue group sample are subtracted with the △ Ct of tumor tissues sample in this experiment, and same
When opposite number is taken to all results, the result which obtains is exactly-△ △ Ct.Finally, p- △ △ Ct carry out 2 power fortune
It calculates, i.e. 2^- △ △ Ct just show that the multiple of expression quantity changes.In triplicate, it is examined using nonparametric t- for statistical analysis.I
Find, the expression quantity of LINC00200 is higher than normal control in the tumor tissues of kidney(See Fig. 1), difference have statistics it is poor
Different (p < 0.05).
6, by 60 patients with renal cell carcinoma follow-up statistics being included in above-mentioned experiment, including patient's First episode when
Between, treatment, recurrence status and death time etc., follow up time is at least 12 months.In selected patients with renal cell carcinoma, choosing
It is reference standard to take the expression value that real-time fluorescence quantitative PCR is analyzed, and the corresponding normal structure of acquired results compares.Tumour
Non-coding RNA LINC00200 expression is defined as non-coding RNA LINC00200 higher than the patient of normal control tissue in tissue
High expression group, remaining is low expression group.By Kaplan-Meier survival analysis, non-coding RNA LINC00200 high expression is suffered from
The life cycle of person is substantially reduced than the patient of non-coding RNA LINC00200 low expression groups, and prognosis is worse(See Fig. 2), difference tool
Have statistically significant (p < 0.05).Therefore, non-coding RNA LINC00200 can be used as the specificity point of prognosis of patients with renal cell carcinoma
Sub- marker.
Sequence table
<110>The first affiliated hospital of Zhengzhou University
<120>Application, kit and the detection method of kidney prognosis novel molecular marker non-coding RNA LINC00200
<141> 2018-04-27
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gcgtagatga gggatggcgc cggcgcaggc ctgcgcgcca cgcgctttag gtggatgagg 120
gatggcgcag gtgcaggcct gcgcgcctca cgctttatgt acatgaggga tgaggcagca 180
caggaattgg cacaacctga agtcagctct gcagctttcc aagcttcgtt ctgcgtgtcc 240
tgtactcaac agtcatctca tgctgcaggg tggctgcgtg tgctccgtac atcacaccca 300
tatttcaggg agaagactgc acatataaca cagctctgca tggaaaacct tccgcctgga 360
ggggtggctt cctagaggtg tggcgttgcc ctctgtcttg aacaggctgt gagccgtttt 420
gtcatttggg gtttctagat gcaaacagca gaagctgctg gccaattacc aaagggaacg 480
tgctgttagg atatcagggc ctgggagctg cagcaatgtg ggctgacagc agagagctaa 540
ggcactttcc gaggtgacga gctgggctgc tatgctggag acggctgggc agaagcagtt 600
agcagggcat ttccttgtgt ccttatctca agagtcacag tttcaggagt gagcatctca 660
gaggtcaggg ttcattcaca tgccacctcc cttctcactg tgtcattggg gaggggccgt 720
ctggaccctc tggctcctgt ggcaagaaat ggtcccatca agtcatccaa gggcctggaa 780
gcctcccaag gaaagcagga gggctgggtg ctgagcagcg tccagcagca aaggtaggct 840
ccagccccgc aggtgtggct gcgccatccc agggaacgtg ccccagcaag tgctggtgct 900
gctctcacta caggtggggt tggtttcact ggacaggtgg cacttcctca cctcttgccc 960
tctggaccca cggcaggcac tttccagggc acatcacgtg ggtgtgcggt ctggctgctg 1020
ggtccacgcg ggttctcaat catgacctgg cttgcaagct ctttccacag ttggataaat 1080
gaagccgttg gggaagtatc cgcaaactct tacagtgagt atgtgataat gacacacgcg 1140
tggcccttct aagacctccg ctaggcatta tcagtgactg tgctcgtgag cgctgacctc 1200
cgctaggcgt tatcagggac tgtgctcgtg agcgccgacc tccgctaggc gttatcaggg 1260
actgtgctcg tgagcgcgga cctccgctag gcgatatcag ggactgtgct catgagggcg 1320
gactttcacc agccacgctt ccgaggagtg gagtctttct cagctctgcc tctccaagat 1380
gaccatcttg tgaagacgat gcgttcttta tacacaagtt ctgtgtgtgt gtgtgtgtgt 1440
tccacacaca ggaccaaagt tgagataggc gcacattttc ttggtcccac ttgtggcccc 1500
agtcggctgt cagaagtggg tgtgctccac atgtacccac catgtcaggg cacagtgctc 1560
acatttcaca cctcagcagg tgccttgatg ttgaccagag gccccaaaat catctctttc 1620
tatgacttct agatcttaga ttcccaggaa ctgggaaatg cagtcagtat cttttgggtc 1680
caagaaactt tgtcagagcc cttgtgggag aaccatagat tctcaccaga taaacagaag 1740
agcttcgtgt tagagaaacc cgcctgtctc cccacattct cagttttctg gagagcagct 1800
gaaagccatc tgggtggaga ttaagagctc caaccgtgta gctttgatgt atcgggcaag 1860
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cttaaagttg tgaggattaa aaacagtaat gaaaagtgag tggcaagtgc cgagtacaca 1980
gtcaagtacc tgatactttt tagtgtaagg taagtagcaa gaaagcatga aatttatttt 2040
catttactct tactacatgt ggtaaaccat ctatgcacag agcactgcat tgggtgccat 2100
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gtgaaagtcc gccctcatga 20
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tggagccctg aatgttgacc 20
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Claims (7)
1. kidney prognosis novel molecular marker non-coding RNA LINC00200 is preparing the preparation of prediction prognosis of patients with renal cell carcinoma
Using the nucleic acid sequence such as SEQ NO of non-coding RNA LINC00200:Shown in 1.
2. the application of kidney prognosis novel molecular marker non-coding RNA LINC00200 according to claim 1, special
Sign is:The preparation for predicting prognosis of patients with renal cell carcinoma is real-time fluorescence quantitative PCR detection kit.
3. a kind of kit as claimed in claim 2, it is characterised in that:Including being used to detect non-coding RNA LINC00200
The nucleic acid sequence of the specific primer of expression, the specific primer is SEQ NO:2 and SEQ NO:3 and reference gene
The nucleic acid sequence of the primer sequence of TUBA1A expression, the primer is SEQ NO:4 and SEQ NO:5.
4. kit according to claim 3, it is characterised in that:Also contain and extracts RNA from tissue and carry out reverse transcription
And all reagents of real-time fluorescence quantitative PCR, including (1) from the tumour of kidney or normal control tissue used in extracted total RNA
Reagent, including Trizol liquid, chloroform, isopropanol, inhibition RNA degradations solvent, 75% ethyl alcohol, DEPC water;(2) using total serum IgE as mould
LINC00200 reverse transcriptions are cDNA agents useful for same by plate, including reverse transcription reaction buffer solution, contain the triphosphoric acid base containing Mg2+
The mixture of deoxynucleotide dNTP, reverse transcriptase M-MLV and random primer and Oligo dT primers;(3) cDNA is real-time
Quantitative PCR agents useful for same, including LINC00200 real-time fluorescence quantitative PCRs specific primer, TUBA1A internal reference specific PCRs draw
Object, real time fluorescent quantitative SYBR dyestuffs, the water without RNA enzyme.
5. the detection method of kidney prognosis novel molecular marker non-coding RNA LINC00200, it is characterised in that:Including with
Lower step:1)Collect kidney to be measured or normal control tissue;
2) extracting of RNA in organizing;
3)The reverse transcription of LINC00200 RNA, using cell total rna as template, reverse transcription obtains cDNA;
4)Using cDNA as template, real-time fluorescence quantitative PCR expansion is carried out using the specific primer of non-coding RNA LINC00200
Increase, detects non-coding RNA LINC00200 expression quantity.
6. the detection method of kidney prognosis novel molecular marker non-coding RNA LINC00200 according to claim 5,
It is characterized in that:Step 3)Middle reverse transcription reaction system is 5 × RT Buffer(Containing Mg2+ and dNTP)4 μ l, 10 × RT
Primer Mix(Oligo dT Primer and Random Hexamers mixtures)2 μ l, BeyoRT II M-MLV are reversed
Record enzyme (RNase H-)(Inhibitor containing RNase)2 μ l, DEPC-treated water, 2 μ l remove the Total after gDNA
RNA 10μl。
7. the detection method of kidney prognosis novel molecular marker non-coding RNA LINC00200 according to claim 5,
It is characterized in that:Step 4)The expression quantity relative quantitation method of middle detection marker non-coding RNA LINC00200.
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