Abstract
PURPOSE: Hypodontia is the congenital absence of one or more (up to six) permanent and/or deciduous teeth, being one of the most common alterations of the human dentition. Genetic polymorphisms are variations of DNA sequences occurring in a population. This study investigated whether G-915C single nucleotide polymorphism (SNPs) in the PAX9 gene promoter is associated with hypodontia in humans. MATERIAL AND METHODS: The polymorphism in region G/C-915 of PAX9 gene (NCBI ref SNP ID: rs 2073247) of 240 patients was analyzed, being 110 controls and 130 individuals with third molar agenesis. After DNA extraction, the region of interest was amplified by PCR technique using two different primers. The significance of the differences in observed frequencies of polymorphisms in both groups was assessed by odds-ratio and chi-squared test with 95% confidence interval. RESULTS: Genotype CC was more frequent in patients with agenesis (11.5%) compared to the control (1.8%), while GG was more prevalent in the control group (39.1%) compared to the individuals with agenesis (26.2%). CONCLUSION: These data showed that the allele C could be associated with the third molar agenesis.
Hypodontia; PAX9 transcription factor; Tooth abnormalities; Genetic polymorphism
ORIGINAL ARTICLES
Association between polymorphism in the promoter region (G/C-915) of PAX9 gene and third molar agenesis
Fabio José BianchI; Tiago Franco de OliveiraII; Cristiane Borges Pereira Saito I ; Regina Célia Rocha Peres III ; Sérgio Roberto Peres Line IV
IDDS, MSc, Postgraduate student, Department of Morphology, Dental School of Piracicaba, State University of Campinas, Piracicaba, SP, Brazil
IIGraduate student, Department of Morphology, Dental School of Piracicaba, State University of Campinas, Piracicaba, SP, Brazil
IIIDDS, MSc, PhD, Assistant Professor, Department of Pediatric Dentistry, Dental School of Piracicaba, State University of Campinas, Piracicaba, SP, Brazil
IVDDS, MSc, PhD, Chair Professor, Department of Morphology, Dental School of Piracicaba, State University of Campinas, Piracicaba, SP, Brazil
Corresponding address Corresponding address: Prof. Dr. Sergio R. P. Line Faculdade de Odontologia de Piracicaba, UNICAMP Avenida Limeira 901, Cx. Postal 51 13414-903 Piracicaba, SP, Brasil Phone: 55 19 2106-5333 e-mail: serglin@fop.unicamp.br or fabiojbianchi@yahoo.com.br
ABSTRACT
PURPOSE: Hypodontia is the congenital absence of one or more (up to six) permanent and/or deciduous teeth, being one of the most common alterations of the human dentition. Genetic polymorphisms are variations of DNA sequences occurring in a population. This study investigated whether G-915C single nucleotide polymorphism (SNPs) in the PAX9 gene promoter is associated with hypodontia in humans.
MATERIAL AND METHODS: The polymorphism in region G/C-915 of PAX9 gene (NCBI ref SNP ID: rs 2073247) of 240 patients was analyzed, being 110 controls and 130 individuals with third molar agenesis. After DNA extraction, the region of interest was amplified by PCR technique using two different primers. The significance of the differences in observed frequencies of polymorphisms in both groups was assessed by odds-ratio and chi-squared test with 95% confidence interval.
RESULTS: Genotype CC was more frequent in patients with agenesis (11.5%) compared to the control (1.8%), while GG was more prevalent in the control group (39.1%) compared to the individuals with agenesis (26.2%).
CONCLUSION: These data showed that the allele C could be associated with the third molar agenesis.
Uniterms: Hypodontia; PAX9 transcription factor; Tooth abnormalities; Genetic polymorphism.
INTRODUCTION
Hypodontia, the congenital absence of one or a few teeth, is one of the most common developmental alterations of human dentition. Hypodontia is not a serious public health problem, but it may cause masticatory (temporomandibular joint disorders) and speech dysfunctions and create esthetic problems with orthodontic and prosthetic impairments29. In the past few years, several growth and transcription factors have been shown to be expressed in developing teeth26. The direct participation of several genes in tooth development was demonstrated by the lack of teeth in mutant knockout mice models7. Autosomal dominant forms of hypodontia have been shown to be caused by mutations in the MSX1 and PAX9 genes in human families25. However, the origin of the isolated sporadic agenesis, the most common form of hypodontia in humans, is still unknown. To date only a limited number of mutations of MSX1 and PAX9 have been proven to be associated with severe hypodontia (oligodontia) in humans11.
PAX9 is a transcription factor that is expressed in dental mesenchyme at initiation, bud, cap and bell stages of odontogenesis15. Protein products of this gene serve as transcription factors that are responsible for the crosstalk between epithelial and mesenchymal tissues and are essential for the establishment of the odontogenic potential of the mesenchyme23,27. It has been found that PAX9-deficient mice lack teeth and pharyngeal pouches derivates and have severe craniofacial anomalies16. The expression of PAX9 in the mesenchyme appears to be a marker for the sites of tooth formation as it occurs before any morphological manifestation of this process12. Mutations in this gene have been shown to be associated with autosomal dominant forms of oligodontia (agenesis of more than 6 teeth, MIM 604625) in humans10,25. In most families, mutations occur in exon 2 affecting the function of PAX9 paired domain that is responsible for the binding of this protein to DNA target sequences. Affected individuals have severe tooth agenesis with absence of most molars, second premolars and some incisors. PAX9 is critical for the regulation of BMP4 expression through its paired domain rather than Msx113.
Polymorphisms are a mechanism by which individuals may exhibit variations within the range of what is considered biologically normal. Gene polymorphisms have also been associated with susceptibility to diseases. Most polymorphisms are single nucleotide exchanges that occur at a high frequency in the human genome and may affect the function of genes. Although it has been demonstrated that mutations in the coding sequences of PAX9 are a causative factor in familiar forms of severe tooth agenesis, polymorphisms in this gene have not been associated with sporadic tooth agenesis.
Previous studies have shown that two polymorphisms in the PAX9 promoter region seem to be associated to the dental agenesis in human beings (G-1031A, T-912C T-160C). The purpose of the present study was to investigate whether the G-915C single nucleotide polymorphism (SNPs) in the PAX9 gene promoter is associated with hypodontia in humans15,22.
MATERIAL AND METHODS
Subject Selection and Sampling
One hundred and thirty unrelated Caucasian individuals with hypodontia, without signs of other disorders and 110 healthy control individuals (without hypodontia) were interviewed and documented. Congenital absence of teeth was confirmed by X-ray examination. No other dental anomalies were observed in the subjects. The sampling of epithelial buccal cells was performed as previously described15. Briefly, individuals undertook a mouthwash of 5 mL 3% glucose. Following mouthwash, a sterile wooden spatula was used to scrape oral mucosa. The tip of the spatula was then shacked into the retained mouthwash solution. Buccal epithelial cells were pelleted by centrifugation at 2000 rpm for 10 min. The supernatant was discarded and the cell pellet resuspended in 500 µL extraction buffer [10 mM Tris-HCl (pH 7.8), 5 mM EDTA, 0.5% SDS]. The samples were then frozen at -20ºC until used for DNA extraction. After defrosted, samples were incubated overnight with 100 ng/mL proteinase K (Sigma Chemical Co., St. Louis, MO, USA) at 37°C with agitation. DNA was then purified by sequential phenol/chloroform extraction and salt/ethanol precipitation. DNA was dissolved in 70 µL TE buffer [10 mM Tris (pH 7.8), 1 mM EDTA]. The concentration was estimated by measurements of OD 26015.
Polymerase Chain Reaction (PCR)
Amplification of the PAX9 gene fragment was performed with the oligonucleotides 5'AGC CTG AAT CCT GTG TGC AC-3' (forward) and two reverses to amplify the region with alleles G or C. To amplify the alelles G the oligonucleotide 5'GAA ATA TTT TCG TGA ATT TGG GAG'-3' was used and the C allele was amplified with the oligonucleotide 5'ATT TTC GTG AAT TTG GGAC'-3' (NCBI ref SNP ID: rs 2073245). Reactions were conducted in a total volume of 50 mL, containing: 10 mM Tris-HCl (pH 8.3), 50 mM KCl, 1 mM of each primer, 200 mM each dATP, dCTP, dGTP and dTTP, 25 mM MgCl2 and 2.5 units Taq DNA polymerase (Amersham Pharmacia Biotech, Uppsala, Sweden). The thermal cycling conditions consisted of an initial denaturation at 95°C for 5 min followed by 35 cycles of 95°C for 60 sec, annealing at 56°C for 70 sec, and a final extension at 72°C for 70 sec. Reactions were performed on a GeneAmp® PCR System 2400 thermocycler (Perkin Elmer).
PCR products of PAX9 were submitted to 10% polyacrylamide gel electrophoresis and the DNA bands were labeled by silver staining15.
Statistical Analysis
The significance of the differences in observed frequencies of polymorphisms in both groups was assessed by odds-ratio and chi-squared test with 95% confidence interval. All statistical analysis was conducted using BioEstat program version 2.0. Differences were considered significant at p<0.0515.
RESULTS
The statistical analysis showed significant differences in the alleles and genotypes frequencies in the promoter polymorphisms of PAX9 gene (G-915C). The C allele was found in 31.4% of the control group and in 42.5% of the test group (individuals with hypodontia) (p=0.0014). The G/G and C/C genotypes frequencies were 39.1% and 1.8% in the control group and 26% and 11.4% in the test group respectively (p=0.0045). The frequencies of different alleles and genotypes of the PAX9 gene are shown in Table 1. The association was confirmed when the CC genotype is confronted with CG/GG. Individuals with CC genotype seemed to be seven times more susceptible to develop hypodontia (OR= 7.04; 95% CI= 1.1-15.2; p= 0.0034).
DISCUSSION
The G-915C polymorphism in the 5' flanking region of PAX9 gene could be associated with hypodontia in humans. CC genotype was found at a significant higher frequency in individuals with hypodontia. Analysis of human families shows a strong effect of PAX9 mutations on third molar agenesis, whereas mutations in this gene have a weaker but fairly evident effect on the development of incisors and premolars.4-6,18-20,24,28. Three other polymorphic alleles (T-160C, G1031A and T912C) located close to the polymorphic region evaluated here were also associated with hypodontia in humans22.
Families bearing PAX9 mutation had tooth agenesis as the only clinical sign. The relative lack of pleiotropy of mutations in PAX9 and on other genes affecting the dental field would account for the common variation in the form and number of teeth observed in humans and other mammals2. This would allow genetic changes to affect the earlier phases of tooth development, without interfering significantly with the development of other organs16.
Experimental and theoretical approaches have stressed the importance of cis-regulatory DNA sequences that control the transcription of genes as the basic modular unit that determine the positional information in developing structures3. The cis-regulatory sequences of many genes are organized into independent modules that regulate the transcription of specific tissues at specific times during development7. The regulatory modules are usually constituted of multiple binding sites for transcription factors that can be located near the transcription start site, or thousand of base pairs away1. Mutations within individual modules can enhance or repress gene transcription in a tissue specific manner, allowing a mutation to exert its effect on a few or even a single morphogenetic field7. A relevant fact is the relative lack of pleiotropic effects of PAX9 gene mutations in humans. Families bearing PAX9 mutation had tooth agenesis as the only clinical sign. The relative lack of pleiotropy of mutations in PAX9 gene and on other genes affecting the dental area would account for the common variation in the form and number of teeth observed in humans and other mammals2. This would allow genetic changes to affect the earlier phases of tooth development, without interfering significantly with the development of other organs.
For example, the down-regulation of Msx1 expression in PAX9-deficient mice and decreased levels of Bmp4 expression in PAX9 and Msx1 homozygous null mice indicate that the three genes act within the same signaling pathway. Although recent studies of human PAX9 mutations have enabled structure-function correlations, the precise molecular mechanisms that contribute to tooth agenesis are poorly understood. The functional studies of a previously described mutation (L21P) in the amino-terminal
subdomain of the PAX9 paired domain demonstrate impaired transcriptional activation of the Msx1 and Bmp4 promoters. It is likely that the proline cyclic side chain blocks the main chain nitrogen atom and chemically prevents it from forming a hydrogen bond13.
In humans, the changes in the number of teeth tend to occur in the reverse of the sequence that teeth are formed during development, which also characterizes the general pattern of tooth loss observed during the evolution of placental mammals17. Variations in tooth number may have represented an important factor in the diversification of mammalian species. Like hypodontia, most evolutionary changes in tooth number resulted from the loss of one or two elements, in most cases the last member of a tooth family. In this regard, the study of genetic polymorphisms in tooth agenesis is a specially suited model to understand the association of gene polymorphisms and changes in morphology. Teeth are serially homologous structures and the effects of gene variations on the development of these structures can be easily quantified8. Individuals with distinct polymorphic alleles may exhibit subtle and specific phenotypic variations in dental patterning. In this sense, association studies between gene polymorphisms and hypodontia as well as other mild malformations that reflect qualitative defects of embryogenesis14, may help understanding the molecular mechanisms responsible for the phenotypic variations that may occur in distinct human populations and ethnic groups.
The first mutation described in human PAX9 gene was an insertion of an additional G within the paired box sequence at nucleotide 219 (219InsG) of exon 2 in a family with oligodontia. Since then eight additional mutations in the coding region of PAX9 gene were reported being associated with oligodontia in humans8. Seven out of the nine reported mutations were located in the paired domain at exon 2. Recently, it has been shown that the 219InsG frameshift mutation dramatically reduces DNA binding of the PAX9 paired domain and supports the hypothesis that loss of DNA binding is the pathogenic mechanism by which the mutation causes oligodontia9. Although mutations in the coding sequences of PAX9 and MSX1 genes are a causative factor in familiar forms of oligodontia6, the genetic origin of the isolated sporadic agenesis, the most common form of hypodontia in humans, is still unknown. We report here that three other polymorphisms (T-160C, G-1031A and T-912C) in the 5' flanking region of PAX9 gene are associated with hypodontia in humans. Other alleles, such as C (-160), A (-1031) and C (-912) were found at a significant higher frequency in individuals with hypodontia. A comparative analysis of mouse, rat and human PAX9 5' flanking sequences shows that the T-160C is located in a poorly conserved region when human and rodent (mice and rat) sequences are compared. Although the present study showed a positive association on genotype and odds ratio, the results must be confirmed by studies with other populations and functional experiments, such as homologous recombination in mice, gel shift analysis and reporter gene systems.
CONCLUSION
The findings of this study showed that the allele C could be associated with third molar agenesis.
Received: January 18, 2007
Modification: March 07, 2007
Accepted: May 29, 2007
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Publication Dates
-
Publication in this collection
06 Nov 2007 -
Date of issue
Oct 2007
History
-
Received
18 Jan 2007 -
Reviewed
07 Mar 2007 -
Accepted
29 May 2007