Qu Yu-jin, Song Fang, Wang Hong, Jin Yu-wei
Department of Medical Genetics, Capital Institute of Pediatrics, Beijing, 100020, P. R. China.
Zhonghua Yi Xue Yi Chuan Xue Za Zhi. 2006 Dec;23(6):680-2.
To establish a single and rapid method for detecting the prevalent mutations of 6-pyruvoyl-tetrahydropterin synthase (PTPS) gene in Chinese patients with 6-pyruvoyl-tetrahydropterin synthase deficiency (PTPSD).
PCR-restriction fragment length polymorphism (PCR-RFLP) was used to detect three prevalent PTPS gene mutations in 4 cases of tetrahydrobiopterin deficiency (BH4D) and their parents, which was performed by the artificial construct restriction site (ACRS). PCR-RFLP included Hpa I digestion for the detection of mutation N52S (155A to G), Hae III for P87S (259C to T) and Eco R I for D96N(286G to A). The mutations of PTPS gene were confirmed by direct sequencing.
The genotypes of 4 PTPS deficient patients were identified: N52S/-, P87S/D96N, N52S/D96N and D96N/-. The result of direct sequencing was coincident with that of PCR-RFLP analysis.
(1) The PCR-RFLP analysis formed by ACRS would be a good way for detecting the three prevalent PTPS gene mutations in Chinese patients with PTPSD. (2)The PTPS gene analysis is very important for all patients with hyperphenylalaninemia, which would be useful for early clinical diagnosis and correct treatment of BH4D patients.
建立一种单一且快速的方法,用于检测中国6-丙酮酰四氢蝶呤合成酶缺乏症(PTPSD)患者中6-丙酮酰四氢蝶呤合成酶(PTPS)基因的常见突变。
采用聚合酶链反应-限制性片段长度多态性(PCR-RFLP)技术,通过人工构建限制性位点(ACRS)检测4例四氢生物蝶呤缺乏症(BH4D)患者及其父母中PTPS基因的三种常见突变。PCR-RFLP包括用Hpa I酶切检测N52S突变(155A→G),用Hae III酶切检测P87S突变(259C→T),用Eco R I酶切检测D96N突变(286G→A)。PTPS基因的突变通过直接测序进行确认。
鉴定出4例PTPS缺乏患者的基因型:N52S/-、P87S/D96N、N52S/D96N和D96N/-。直接测序结果与PCR-RFLP分析结果一致。
(1)由ACRS构成的PCR-RFLP分析是检测中国PTPSD患者中三种常见PTPS基因突变的良好方法。(2)PTPS基因分析对所有高苯丙氨酸血症患者都非常重要,这将有助于BH4D患者的早期临床诊断和正确治疗。
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