Font-Llitjós Mariona, Rodríguez-Santiago Benjamín, Espino Meritxell, Sillué Ruth, Mañas Sandra, Gómez Laia, Pérez-Jurado Luis A, Palacín Manuel, Nunes Virginia
Medical and Molecular Genetics Center, IDIBELL, Hospital Duran i Reynals, L'Hospitalet de Llobregat, Barcelona, Spain.
Eur J Hum Genet. 2009 Jan;17(1):71-9. doi: 10.1038/ejhg.2008.145. Epub 2008 Aug 20.
Lysinuric protein intolerance (LPI) is a rare autosomal inherited disease caused by defective cationic aminoacid transport 4F2hc/y(+)LAT-1 at the basolateral membrane of epithelial cells in the intestine and kidney. LPI is a multisystemic disease with a variety of clinical symptoms such as hepatosplenomegaly, osteoporosis, hypotonia, developmental delay, pulmonary insufficiency or end-stage renal disease. The SLC7A7 gene, which encodes the y(+)LAT-1 protein, is mutated in LPI patients. Mutation analysis of the promoter localized in intron 1 and all exons of the SLC7A7 gene was performed in 11 patients from 9 unrelated LPI families. Point mutation screening was performed by exon direct sequencing and a new multiplex ligation probe amplification (MLPA) assay was set up for large rearrangement analysis. Eleven SLC7A7-specific mutations were identified, seven of them were novel: p.L124P, p.C425R, p.R468X, p.Y274fsX21, c.625+1G>C, DelE4-E11 and DelE6-E11. The novel large deletions originated by the recombination of Alu repeats at introns 3 and 5, respectively, with the same AluY sequence localized at the SLC7A7 3' region. The novel MLPA assay is robust and valuable for LPI molecular diagnosis. Our results suggest that genomic rearrangements of SLC7A7 play a more important role in LPI than has been reported, increasing the detection rate from 5.1 to 21.4%. Moreover, the 3' region AluY repeat could be a recombination hot spot as it is involved in 38% of all SLC7A7 rearranged chromosomes described so far.
赖氨酸尿性蛋白不耐受症(LPI)是一种罕见的常染色体隐性遗传病,由肠道和肾脏上皮细胞基底外侧膜上的阳离子氨基酸转运体4F2hc/y(+)LAT-1缺陷引起。LPI是一种多系统疾病,有多种临床症状,如肝脾肿大、骨质疏松、肌张力减退、发育迟缓、肺功能不全或终末期肾病。编码y(+)LAT-1蛋白的SLC7A7基因在LPI患者中发生突变。对来自9个无关LPI家族的11名患者进行了SLC7A7基因内含子1中的启动子及所有外显子的突变分析。通过外显子直接测序进行点突变筛查,并建立了一种新的多重连接探针扩增(MLPA)检测方法用于大片段重排分析。共鉴定出11种SLC7A7特异性突变,其中7种为新突变:p.L124P、p.C425R、p.R468X、p.Y274fsX21、c.625+1G>C、DelE4-E11和DelE6-E11。这些新的大片段缺失分别由内含子3和5处的Alu重复序列与位于SLC7A7 3'区域的相同AluY序列重组产生。这种新的MLPA检测方法对于LPI的分子诊断是可靠且有价值的。我们的结果表明,SLC7A7的基因组重排在LPI中所起的作用比之前报道的更为重要,将检测率从5.1%提高到了21.4%。此外,3'区域的AluY重复序列可能是一个重组热点,因为在目前描述的所有SLC7A7重排染色体中,有38%涉及该序列。