概要

A Method to Study the C924T Polymorphism of the Thromboxane A2 Receptor Gene

Published: April 01, 2019
doi:

概要

In the present study, we describe a methodology to analyze the C924T genotype. The protocol consists of three phases: DNA extraction, amplification by polymerase chain reaction (PCR), and analysis of the restriction fragment length polymorphism (RFLP) on agarose gel.

Abstract

The thromboxane A2 receptor (TBXA2R) gene is a member of the G-protein coupled superfamily with seven-transmembrane regions. It is involved in atherogenesis progression, ischemia, and myocardial infarction. Here we present a methodology of patient genotyping to investigate the post-transcriptional role of the C924T polymorphism (rs4523) situated at the 3' region of the TBXA2 receptor gene. This method relies on DNA extraction from whole blood, polymerase chain reaction (PCR) amplification of the TBXA2 gene portion containing the C924T mutation, and identification of wild type and/or mutant genotypes using a restriction digest analysis, specifically a restriction fragment length polymorphism (RFLP) on agarose gel. In addition, the results were confirmed by sequencing the TBXA2R gene. This method features several potential advantages, such as high efficiency and the rapid identification of the C924T polymorphism by PCR and restriction enzyme analysis. This approach allows a predictive study for plaque formation and atherosclerosis progression by analyzing patient genotypes for the TBXA2R C924T polymorphism. Application of this method has the potential to identify subjects who are more susceptible to atherothrombotic processes, in particular subjects in a high-risk, aspirin-treated group.

Introduction

TBXA2R is a member of the G-protein coupled superfamily with seven-transmembrane regions, which are widely expressed and localized either on the cell membranes or on intracellular structures1,2. The TBXA2R signaling pathway is involved in advanced atherosclerotic processes3. Increased expression of the TBXA2 receptor was demonstrated during the atherogenesis progression, and clinical and experimental studies showed its relevant role in ischemia and myocardial infarction4. C924T, a single nucleotide polymorphism (SNP) of the TBXA2R gene, was recognized as a functional polymorphism in healthy volunteers and has been linked to clinical disorders5. Furthermore, our previous study6 demonstrated that the C924T polymorphism of the TBXA2R gene is involved in transcript stability; specifically, there is an increased instability of the mutant (TT) type transcript with respect to the wild type (CC). In addition, several stimuli such as adenosine diphosphate (ADP), epinephrine, and collagen at different concentrations induced a platelet aggregation less effective for the mutant type (TT). This is consistent with a reduced thrombus formation and hemostasis. Thus, the instability of the TBXA2R transcript and the associated reduction of platelet aggregation might be associated with a protective role for the TBXA2R TT genotype against atherothrombosis and its complications in high-risk aspirin-treated patients6.

Here, we describe a methodology for patient genotyping to investigate the post-transcriptional role of C924T polymorphism (rs4523) situated at the 3' region of the TBXA2 receptor gene. This method relies on the following steps: (1) DNA extraction from whole blood, (2) PCR amplification of the TBXA2R gene portion containing the C924T mutation, and (3) identification of wild type and/or mutant genotypes using restriction fragment length polymorphism (RFLP) on agarose gel. RFLP is a technique that exploits variations in homologous DNA sequences7. This application was used to detect DNA polymorphisms, especially SNPs, and to find and associate biological relevance in genetic variations8. The polymorphism analyzed for the first time using the RFLP-PCR in humans was the ABO blood9. The RFLP-PCR method allows the analysis of genetic mutations in homologous DNA sequences by evaluating the presence of fragments of different lengths after the DNA digestion using highly specific restriction endonucleases10.

In past years, the following methodologies have been utilized for SNP analysis using the PCR technique: hybridization of short allele-specific oligonucleotides11, allele-specific PCR12, primer extension on DNA microarrays13, oligonucleotide ligation assay14, Direct DNA sequencing for identifying position-specific single-nucleotide polymorphisms15, Taqman method16, extraction Matrix-Assisted Laser Desorption/Ionization Time-Of-Flight (MALDI-TOF) mass spectrometry17, and GeneChips18. These techniques are not simple to use and may require expensive equipment. Conversely, the PCR-RFLP method is inexpensive, simple to use, convenient, has a high efficiency, and allows rapid identification of the C924T polymorphism. In addition, we confirmed the results by sequencing the TBXA2R gene using the Sanger method15.

This approach allows a predictive study of plaque formation and atherosclerosis progression by analyzing patient genotypes for the TBXA2R C924T polymorphism. This method could identify subjects more susceptible to atherothrombotic processes, in particular those among high-risk, aspirin-treated patients.

Protocol

The protocol follows the guidelines of the Medical Research Ethics Committee of the University of Chieti.

1. Reagent Setup

  1. Prepare the Tris-EDTA (TE) buffer (pH 8.0). Add 200 µL of EDTA 0.5 M and 1 mL of Tris-Cl 1 M in a beaker and bring to 100 mL with sterile water. TE buffer final concentration: 10 mM Tris-Cl, 1 mM EDTA. Store at room temperature (RT).
  2. Prepare 1 L of the 10x stock solution electrophoresis buffer (TBE). Dissolve 108 g of Tris Base, 55 g of boric acid, and 40 mL of EDTA 0.5 M (pH 8) into a beaker, and bring to volume of 1 L with sterile water. Store at RT.
  3. Prepare the gel loading dye. Dissolve 0.25 g of bromophenol blue, 0.25 g of xylene cyanol FF, 50 g of glycerol, 1 mM of EDTA (pH 8) in 60 mL deionized or distilled water, and bring to a volume of 100 mL with sterile water. Store at 4 °C (for a few months) or at -20 °C (for years)
  4. Prepare 200 mL of 2% agarose gel. Use it fresh or, alternatively, store solidified at RT for up to several weeks.
    1. Dissolve 4 g of agarose in 200 mL of 1x TBE buffer in a 600 mL beaker. Stir using a magnetic mixer for about 5 min until the agarose is completely suspended.
    2. Heat the 2% agarose solution in boiling-water or on a hot plate (for about 10 min, until the agarose is completely dissolved). Note that the beaker with the agarose gel must be covered with aluminum foil. Alternatively, heat the uncovered beaker in a microwave at a high temperature for about 3–5 min.
    3. Swirl the 2% agarose solution using a magnetic mixer, checking that the agarose is completely dissolved.
      NOTE: Particles of agarose appear as translucent grains prior to complete dissolution. It may be necessary to reheat particles for several minutes (about 5–10 min).
    4. If a stored portion of the agarose gel is used, heat the beaker, covered with aluminum foil, in a hot-water bath (at about 60 °C) until the agarose is dissolved. Remove with a Pasteur pipette any "trace" of solidified agarose from the surface prior to pouring.

2. DNA Purification

  1. Perform the following before starting the purification:
    1. Use human fresh whole blood samples, or thaw whole blood frozen samples quickly (for about 2–3 min) in a water bath (at 37 °C) applying a mild agitation and then equilibrate to RT before use.
    2. Mix fresh or thawed blood samples inverting the tubes several times.
  2. Start the purification procedure by following the supplier's protocols for 100 µL of elution volume.
  3. Quantify and calculate the purity of DNA measuring the absorbance at 260, 280, and 320 nm.
    1. Use sterile water to dilute the samples and to calibrate the spectrophotometer.
    2. Apply the following formula, in order to calculate the concentration of DNA sample = 50 µg/mL x (A260 − A320) x dilution factor, and the purity of DNA = (A260 − A320)/(A280 − A320), with an acceptable ratio between 1.7 and 1.9.

3. PCR Amplification of DNA Samples

  1. Prepare 25 µL of reaction mixture in a 0.2 mL micro-amplification tube, as shown in Table 1.
  2. Carry out a PCR-amplification of the purified DNA samples using an automated thermal cycler, following the amplification program shown in Table 2.
  3. At the end of the PCR amplification, stop the PCR reactions by leaving the DNA samples at 4 °C.

4. RFLP of PCR Products

  1. Prepare 22.5 µL of master-mix solution for each sample, so that the selected restriction enzyme digests the PCR products, as shown in Table 3.
  2. Transfer 2.5 µL of PCR product to a new PCR tube for each sample, using a pipette and filter tips.
  3. Add 22.5 µL of digestion master-mix solution to the tubes containing the PCR product of each sample, using a pipette and filter tips.
  4. Incubate the reaction mixture (master-mix solution and PCR product) at 37 °C for 4 h.

5. Gel Electrophoresis Analysis of PCR-RFLP Samples

  1. Stain the agarose gel by adding ethidium bromide (EtBr) at 0.5 µg/mL to the gel for 10 min. EtBr binds to the DNA, which can be visualized under ultraviolet (UV) light.
    Caution: It is important to use gloves and other protective devices during handling, storage, and disposal of EtBr, because it is a mutagen with potential carcinogenicity.
  2. Pour the prepared agarose gel into a gel tray with the well comb in place, and wait until it is solidified.
  3. Place the solidified agarose gel into the gel box (electrophoresis unit).
  4. Fill the gel box with 1x TBE until the gel is covered.
  5. With a pipette and filter tips, load 6 µL of the amplified digest DNA (specifically, load 5 µL of each sample and 1 µL of gel loading dye) into the wells of the agarose gel. Add a DNA size marker in a separate well and in parallel with the samples.
  6. Run the gel for 20–30 min at 100 V.
  7. With a UV-transilluminator, visualize the cleaved DNA fragments or the undigested PCR products, comparing fragments with the DNA size marker, and register the results by photography following the manufacturer's instructions.
    Caution: Use protective devices (safety glasses or a face mask) around UV light sources.

Representative Results

The goal of this method is to evaluate the Thromboxane A2 receptor genotype with regard to the C924T polymorphism. The human TBXA2R gene is located on 19p13.3, spans 15 kbp, and consists of three exons separated by two introns. The C924T polymorphisms of the TBXA2R gene (of 539 bp) was amplified using the PCR primers shown in Figure 1, which were well-engineered to amplify a specific DNA region but not an orthologous or paralogous nonspecific region. In addition, an RFLP analysis using an RsaI restriction enzyme (Figure 1) on the PCR products was performed and the results were visualized on an agarose gel, in order to characterize the specific studied SNP.

Based on the presence of different fragment lengths after digestion of the DNA, it is possible to discriminate a patient's genotype for the C924T polymorphism. In fact, as shown on Figure 2, the homozygosity of the major allele (CC) displays two bands (395 and 144 bp), because the restriction enzyme precisely cuts the TBXA2R gene portion at the C924T polymorphism site. The homozygosity of the minor allele (TT) is demonstrated by a single band (539 bp), because the restriction enzyme cutting does not occur. The heterozygous (CT) allele shows three bands (539, 395, and 144 bp). As shown in Figure 2, the C924T polymorphism, defined by RsaI digestion on PCR product, has been confirmed by sequence analysis.

Component Volume (µL) Final concentration
10x PCR buffer Tween-20 (15 M MgCl2) 0.25 1.5 MgCl2 mmol/L
dNTP mix (10 mM) 1 200 µM
Primer (forward)(10 pmol/µM) 1 0.4 µM/µL
Primer (reverse)(10 pmol/µM) 1 0.4 µM/µL
Taq polymerase (5 U/µL) 0.2 1 U/µL
Sample DNA (42 ng/µL) 1 42 ng/µL
DNase-free-water 20.55
Total 25

Table 1: PCR amplification setup. A 25 µL master-mix reaction mixture set up in a 0.2 mL PCR tube to amplify a single DNA sample.

Standard PCR
Initial activating step 5 min 95 °C
3-step cycling
Denaturation 30 s 94 °C
Annealing 60 s 55 °C
Extension 60 s 72 °C
Number of cycles 30 cycles
Final extension 8 min 72 °C

Table 2: PCR amplification program. Set up an automated thermal cycler in order to perform PCR and amplify the template DNA. PCR reactions are stopped by chilling at 4 °C.

Component Volume (µL) (n = 1) Volume (µL) (n = 10)*
10x enzyme buffer 2.5 27.5
Restriction enzyme (5 U/µL) 0.5 5.5
DNase-free-water 19.5 214.5
Total 22.5 247.5

Table 3: Restriction enzyme digestion of PCR products. A master-mix solution is prepared so that the selected restriction enzyme digests the PCR products. *: To set up a master-mix solution for 10 samples, add 10% more, finally making up 11 samples.

Figure 1
Figure 1: PCR primers and RsaI restriction enzyme. The forward and reverse primers designed for amplifying the TBXA2R gene portion of 539 bp containing the C924T polymorphism. RsaI is the restriction enzyme selected to recognize the GTAC sites. ˅: cutting site of RsaI enzyme. C(/T): C924T polymorphism. Please click here to view a larger version of this figure.

Figure 2
Figure 2: Electrophoretic pattern and DNA sequence analysis. (A) The C924T genotype is recognized by the RFLP pattern after digestion with the specific RsaI enzyme. (B) DNA sequence analysis: The results obtained by RFLP after digestion with the RsaI restriction enzyme were confirmed using sequence analysis showing the C924T polymorphism. This figure has been modified from De Iuliis et al., Prostaglandins & Other Lipid Mediators6. Please click here to view a larger version of this figure.

Discussion

In the present study, we have described a methodology that allows patient genotyping in order to investigate the post-transcriptional role of C924T polymorphism (rs4523) situated at the 3' region of the TBXA2R gene. First, this method relies on DNA extraction from whole blood. In particular, this first process consists of a purification of total human DNA, genomic and mitochondrial, from whole blood samples fresh or frozen, treated with EDTA (either citrate or heparin). For short term storage of whole blood samples, store at 2-8 °C for up to 10 days. For storage over 10 days, store samples at -70 °C. The automated purification process comprises 4 steps: lyse, bind, wash, and elute. Second, the method relies on PCR amplification of the TBXA2R gene portion containing the C924T mutation. Finally, identification of the wild type and/or mutant genotype using a restriction enzyme analysis (RFLP) on agarose gel is performed.

Critical steps in the protocol are the following: (i) In the case that a portion of the agarose gel stored at RT is used, the solidified agarose can be re-dissolved over a boiling-water bath (at 60 °C for about 15-20 min) or in a microwave oven (3-5 min) prior to pouring. Note: loosen the cap when re-melting agarose in a bottle. (ii), furthermore, when re-heating agarose, evaporation will cause an increase of its concentration. For this reason, it could be useful to compensate by adding a small volume of water. (iii) DNA fragments of less than 1,000 bp were differentiated by agarose gel, and TBE buffer is recommended to obtain the best possible separation. (iv) We prefer to use an agarose gel rather than a polyacrylamide gel because the preparation of the latter is more difficult, and it takes much longer to set up. (v) The choice of the running time of the gel electrophoresis relies on the expected size of the amplification products. Based on this protocol, it is sufficient to perform an electrophoresis for 20-30 min at 100 V in 2% agarose gel, since the size of the PCR fragments ranges from 100-500 bp. (vi) It is mandatory to obtain 10 to 50 ng of a good quality template DNA extracted from human samples. For this reason, we prefer to use an automated DNA purification rather than a semi-automated or manual one. (vii) Prepare the master-mix reaction for PCR amplification and the master-mix solution for PCR products digestion, adding 10% more (to account for loss of liquid during pipetting) to the volume calculated multiplied by the number of samples for the volume required for one DNA sample.

The most frequent pitfall of the method is the presence of extra amplification products due to an incorrect thermal cycler program, an incorrect amplification master-mix preparation, or a DNA template contamination. Furthermore, the absence of PCR products may be due to inactivated Taq polymerase or an incorrect thermal cycler run. In addition, the presence of unexpected fragments may be due to PCR product contamination or to an incomplete digestion from either an inactivated enzyme, too little amount of restriction enzyme volume, or a too short incubation time.

In the past years, the following methodologies have been utilized for SNP analysis using the PCR technique: hybridization of short allele-specific oligonucleotides11, allele-specific PCR12, primer extension on DNA microarrays13, oligonucleotide ligation assay14, Direct DNA sequencing for identifying position-specific single-nucleotide polymorphisms15, Taqman method16, extraction Matrix-Assisted Laser Desorption/Ionization Time-Of-Flight (MALDI-TOF) mass spectrometry17, and GeneChips18. These methods are not ideal because they are not simple to use and/or require expensive equipment. Conversely, the PCR-RFLP method described in this study is inexpensive, simple to use, convenient, has a high efficiency, and allows rapid identification of the C924T polymorphism. A limitation to the present method is that it can only be used for a small number of SNPs and for a few samples in a working session.

For future applications, this method can be used for predictive studies concerning plaque formation and atherosclerosis progression by analyzing the patient genotypes for the TBXA2R C924T polymorphism. Furthermore, this method could identify subjects more susceptible to atherothrombotic processes, in particular, high-risk patients treated with aspirin. Finally, this method could be applied to study other polymorphisms involved in personalized medicine for specific drugs (for example, anticoagulants and anticonvulsants) in order to understand the appropriate drug dosage and the individual pharmacological and clinical response for each patient before beginning therapy and to avoid adverse effects.

開示

The authors have nothing to disclose.

Acknowledgements

This project was partially funded by 60% Ateneo grants from Ministero dell'Università, Italy to S.M., and E.T. We also received partial contributions to research expenses by the Department of Medical, Oral and Biotechnological Sciences, University of Chieti "G. d'Annunzio".

Materials

QIAsymphony SP QIAGEN 937055
Spectrophotometer EPPENDORF 6131-02222
UV-transilluminator UVP 732-110
PCR tubes EPPENDORF H0030121589
PCR thermal cycler EPPENDORF 5331-03721
Pipettors and filter tips EPPENDORF H4910000018/42/69 AND 0030067037/10/02
Horizontal minigel electrophoresis apparatus DIATECH PHORESIS 10 RI002-10
Dry block heater TWIN INCUBATOR DG210
QIAsymphony DNA Midi Kit QIAGEN 931255
10X PCR buffer (usually supplied by the manufacturer with the Taq polymerase) DIATECH AND TAKARA T0100 AND R0001DM
Taq polymerase TAKARA R0001DM
dNTP mixture DIATECH  pharmacogenetics NM001 dNTP MIX 10X 100 microliters, 10mM
PCR primers DIATECH  pharmacogenetics \
Restriction enzyme RsaI New England biolabs R0167L
Restriction enzyme 10X buffer New England biolabs R0167L
Agarose Sigma A9539 DNA fragments are best separated in TBE buffer
Tris base Sigma T6066
Boric acid Sigma B7901
0.5 M EDTA, pH 8.0 Sigma E7889
10% (wt/vol) ammonium persulfate Sigma E3678 prepared fresh each time
EtBr (0.5 μg/μL) Sigma E8751
Bromophenol blue Sigma B0126
Xylene cyanol FF Sigma X4126
Glycerol Sigma G5516
DNA size marker DIATECH  pharmacogenetics R1002-10 Plasmide pBluescript II SK (+) restrict MSPI
Sterile water (autoclaved) DIATECH  pharmacogenetics \

参考文献

  1. Shen, R. F., Tai, H. H. Thromboxanes: synthase and receptors. J Biomed Sci. 5 (3), 153-172 (1998).
  2. Nusing, R. M., Hirata, M., Kakizuka, A., Eki, T., Ozawa, K., Narumiya, S. Characterization and chromosomal mapping of the human thromboxane A2 receptor gene. J Biol Chem. 268 (33), 25253-25259 (1993).
  3. Cyrus, T., Ding, T., Praticò, D. Expression of thromboxane synthase, prostacyclin synthase and thromboxane receptor in atherosclerotic lesions: correlation with plaque composition. Atherosclerosis. 208 (2), 376-381 (2010).
  4. Cipollone, F., et al. A Polymorphism in the Cyclooxygenase 2 Gene as an Inherited Protective Factor Against Myocardial Infarction and Stroke. JAMA. 291 (18), 2221-2228 (2004).
  5. Fontana, P., et al. Identification of functional polymorphisms of the thromboxane A2 receptor gene in healthy volunteers. Thromb Haemost. 96 (3), 356-360 (2006).
  6. De Iuliis, V., et al. Differential TBXA2 receptor transcript stability is dependent on the C924T polymorphism. Prostaglandins Other Lipid Mediat. pii. (17), (2017).
  7. Saiki, R. K., et al. Enzymatic amplification of beta-globin genomic sequences and restriction site analysis for diagnosis of sickle cell anemia. Science. 230 (4732), 1350-1354 (1985).
  8. Collins, F. S., Brooks, L. D., Chakravarti, A. A DNA polymorphism discovery resource for research on human genetic variation. Genome Res. 8 (12), 1229-1231 (1998).
  9. Lee, J. C. -. I., Chang, J. -. G. ABO genotyping by polymerase chain reaction. J. Forensic Sci. 37 (5), 1269-1275 (1992).
  10. Masao, O., Hirofumi, F., Jerzy, K. K., Hidetoshi, I. Single nucleotide polymorphism detection by polymerase chain reaction-restriction fragment length polymorphism. Nature Protocols. 2 (11), 2857-2864 (2007).
  11. Iwasaki, H., et al. Accuracy of genotyping for single nucleotide polymorphisms by a microarray-based single nucleotide polymorphism typing method involving hybridization of short allele-specific oligonucleotides. DNA Res. 9 (2), 59-62 (2002).
  12. Papp, A. C., Pinsonneault, J. K., Cooke, G., Sadee, W. Single nucleotide polymorphism genotyping using allele-specific PCR and fluorescence melting curves. Biotechniques. 34 (5), 1068-1072 (2003).
  13. O’Meara, D., Ahmadian, A., Odeberg, J., Lundeberg, J. SNP typing by apyrase-mediated allele-specific primer extension on DNA microarrays. Nucleic Acids Res. 30 (15), e75 (2002).
  14. Pickering, J. Integration of DNA ligation and rolling circle amplification for the homogeneous, end-point detection of single nucleotide polymorphisms. Nucleic Acids Res. 30 (12), e60 (2002).
  15. Chatterjee, P. D. Direct sequencing of bacterial and P1 artificial chromosome-nested deletions for identifying position-specific single-nucleotide polymorphisms. Proc. Natl. Acad. Sci. USA. 96 (23), 13276-13281 (1999).
  16. Livak, K. J. Allelic discrimination using fluorogenic probes and the 5′ nuclease assay. Genet. Anal. 14 (5-6), 143-149 (1999).
  17. Haff, L. A., Smirnov, I. P. Single-nucleotide polymorphism identification assays using a thermostable DNA polymerase and delayed extraction MALDI-TOF mass spectrometry. Genome Res. 7 (4), 378-388 (1997).
  18. Gunderson, K. L., Steemers, F. L., Lee, G., Mendoza, L. G., Chee, M. A genome-wide scalable SNP genotyping assay using microarray technology. Nat. Genet. 37 (5), 549-554 (2005).

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記事を引用
De Iuliis, V., Ursi, S., Pennelli, A., Caruso, M., Capodifoglio, S., Marino, A., Flati, V., Vitullo, G., Toniato, E., Robuffo, I., Martinotti, S. A Method to Study the C924T Polymorphism of the Thromboxane A2 Receptor Gene. J. Vis. Exp. (146), e57289, doi:10.3791/57289 (2019).

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