Fabiana H G Farias, Tendai Mhlanga-Mutangadura, Juyuan Guo, Liz Hansen, Gary S Johnson, Martin L Katz
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A study was therefore undertaken to identify the molecular genetic basis of the disease so that dogs could be screened prior to breeding in order to avoid generating affected offspring. <b>Methods:</b> Linkage analysis within a large family of Basenjis that included both affected and unaffected individuals was performed to localize the causative variant within the genome. Significant linkage was identified between chromosome 3 (CFA3) makers and the disease phenotype. Fine mapping restricted the region to a 2.7 Mb section of CFA3. A whole genome sequence of a Basenji affected with Fanconi syndrome was generated, and the sequence data were examined for the presence of potentially deleterious homozygous variants within the mapped region. <b>Results:</b> A homozygous 317 bp deletion was identified in the last exon of <i>FAN1</i> of the proband. 78 Basenjis of known disease status were genotyped for the deletion variant. Among these dogs, there was almost complete concordance between genotype and phenotype. The only exception was one dog that was homozygous for the deletion variant but did not exhibit signs of Fanconi syndrome. <b>Conclusions:</b> These data indicate that the disorder is very likely the result of FAN1 deficiency. The mechanism by which this deficiency causes the disease signs remains to be elucidated. FAN1 has endonuclease and exonuclease activity that catalyzes incisions in regions of double-stranded DNA containing interstrand crosslinks. FAN1 inactivation may cause Fanconi syndrome in Basenjis by sensitization of kidney proximal tubule cells to toxin-mediated DNA crosslinking, resulting in the accumulation of genomic and mitochondrial DNA damage in the kidney. Differential exposure to environmental toxins that promote DNA crosslink formation may explain the wide age-at-onset variability for the disorder in Basenjis.</p>","PeriodicalId":12688,"journal":{"name":"Genes","volume":"15 11","pages":""},"PeriodicalIF":2.8000,"publicationDate":"2024-11-14","publicationTypes":"Journal Article","fieldsOfStudy":null,"isOpenAccess":false,"openAccessPdf":"https://www.ncbi.nlm.nih.gov/pmc/articles/PMC11593659/pdf/","citationCount":"0","resultStr":"{\"title\":\"<i>FAN1</i> Deletion Variant in Basenji Dogs with Fanconi Syndrome.\",\"authors\":\"Fabiana H G Farias, Tendai Mhlanga-Mutangadura, Juyuan Guo, Liz Hansen, Gary S Johnson, Martin L Katz\",\"doi\":\"10.3390/genes15111469\",\"DOIUrl\":null,\"url\":null,\"abstract\":\"<p><p><b>Background:</b> Fanconi syndrome is a disorder of renal proximal tubule transport characterized by metabolic acidosis, amino aciduria, glucosuria, and phosphaturia. There are acquired and hereditary forms of this disorder. A late-onset form of Fanconi syndrome in Basenjis was first described in 1976 and is now recognized as an inherited disease in these dogs. In part because of the late onset of disease signs, the disorder has not been eradicated from the breed by selective mating. A study was therefore undertaken to identify the molecular genetic basis of the disease so that dogs could be screened prior to breeding in order to avoid generating affected offspring. <b>Methods:</b> Linkage analysis within a large family of Basenjis that included both affected and unaffected individuals was performed to localize the causative variant within the genome. Significant linkage was identified between chromosome 3 (CFA3) makers and the disease phenotype. Fine mapping restricted the region to a 2.7 Mb section of CFA3. A whole genome sequence of a Basenji affected with Fanconi syndrome was generated, and the sequence data were examined for the presence of potentially deleterious homozygous variants within the mapped region. <b>Results:</b> A homozygous 317 bp deletion was identified in the last exon of <i>FAN1</i> of the proband. 78 Basenjis of known disease status were genotyped for the deletion variant. Among these dogs, there was almost complete concordance between genotype and phenotype. The only exception was one dog that was homozygous for the deletion variant but did not exhibit signs of Fanconi syndrome. <b>Conclusions:</b> These data indicate that the disorder is very likely the result of FAN1 deficiency. The mechanism by which this deficiency causes the disease signs remains to be elucidated. FAN1 has endonuclease and exonuclease activity that catalyzes incisions in regions of double-stranded DNA containing interstrand crosslinks. 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引用次数: 0
摘要
背景:范可尼综合征是一种以代谢性酸中毒、氨基酸尿、葡萄糖尿和磷酸盐尿为特征的肾近曲小管转运障碍。这种疾病有获得性和遗传性之分。1976 年首次描述了巴仙吉犬的晚发性范可尼综合征,现在这种疾病已被认为是遗传性疾病。由于发病较晚,这种疾病一直未能通过选择性交配从该犬种中根除。因此,我们开展了一项研究,以确定该疾病的分子遗传基础,从而在繁殖前对犬只进行筛查,避免产生患病的后代。研究方法在一个包括患病和未患病个体的巴森吉犬大家族中进行了连锁分析,以确定基因组中的致病变体。结果发现,3 号染色体(CFA3)制造商与疾病表型之间存在显著的关联。精细作图将该区域限制在 CFA3 的 2.7 Mb 部分。研究人员生成了一只患有范可尼综合征的巴仙吉犬的全基因组序列,并对序列数据进行了检验,以确定在映射区域内是否存在潜在的有害同源变异。结果发现在该病例的 FAN1 最后一个外显子中发现了一个 317 bp 的同源缺失。对 78 只已知疾病状态的巴森吉犬进行了缺失变异基因分型。在这些狗中,基因型和表型几乎完全一致。唯一例外的是,有一只狗是缺失变体的同卵双生体,但没有表现出范可尼综合征的症状。结论:这些数据表明,这种疾病很可能是 FAN1 缺乏所致。这种缺陷导致疾病征兆的机制仍有待阐明。FAN1 具有内切酶和外切酶活性,能催化含有链间交联的双链 DNA 区域的切割。FAN1 失活可能会导致肾近曲小管细胞对毒素介导的 DNA 交联敏感,从而导致肾脏中基因组和线粒体 DNA 损伤的积累,从而引起巴仙吉犬的范可尼综合征。不同的环境毒素会促进 DNA 交联的形成,这可能是巴森吉犬发病年龄差异较大的原因。
FAN1 Deletion Variant in Basenji Dogs with Fanconi Syndrome.
Background: Fanconi syndrome is a disorder of renal proximal tubule transport characterized by metabolic acidosis, amino aciduria, glucosuria, and phosphaturia. There are acquired and hereditary forms of this disorder. A late-onset form of Fanconi syndrome in Basenjis was first described in 1976 and is now recognized as an inherited disease in these dogs. In part because of the late onset of disease signs, the disorder has not been eradicated from the breed by selective mating. A study was therefore undertaken to identify the molecular genetic basis of the disease so that dogs could be screened prior to breeding in order to avoid generating affected offspring. Methods: Linkage analysis within a large family of Basenjis that included both affected and unaffected individuals was performed to localize the causative variant within the genome. Significant linkage was identified between chromosome 3 (CFA3) makers and the disease phenotype. Fine mapping restricted the region to a 2.7 Mb section of CFA3. A whole genome sequence of a Basenji affected with Fanconi syndrome was generated, and the sequence data were examined for the presence of potentially deleterious homozygous variants within the mapped region. Results: A homozygous 317 bp deletion was identified in the last exon of FAN1 of the proband. 78 Basenjis of known disease status were genotyped for the deletion variant. Among these dogs, there was almost complete concordance between genotype and phenotype. The only exception was one dog that was homozygous for the deletion variant but did not exhibit signs of Fanconi syndrome. Conclusions: These data indicate that the disorder is very likely the result of FAN1 deficiency. The mechanism by which this deficiency causes the disease signs remains to be elucidated. FAN1 has endonuclease and exonuclease activity that catalyzes incisions in regions of double-stranded DNA containing interstrand crosslinks. FAN1 inactivation may cause Fanconi syndrome in Basenjis by sensitization of kidney proximal tubule cells to toxin-mediated DNA crosslinking, resulting in the accumulation of genomic and mitochondrial DNA damage in the kidney. Differential exposure to environmental toxins that promote DNA crosslink formation may explain the wide age-at-onset variability for the disorder in Basenjis.
期刊介绍:
Genes (ISSN 2073-4425) is an international, peer-reviewed open access journal which provides an advanced forum for studies related to genes, genetics and genomics. It publishes reviews, research articles, communications and technical notes. There is no restriction on the length of the papers and we encourage scientists to publish their results in as much detail as possible.
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