极长链酰基辅酶 A 脱氢酶缺乏症的分子和细胞病理学。
Molecular and cellular pathology of very-long-chain acyl-CoA dehydrogenase deficiency.
机构信息
Department of Pediatrics, University of Pittsburgh School of Medicine, University of Pittsburgh, Children's Hospital of Pittsburgh of UPMC, 4401 Penn Avenue, Pittsburgh, PA 15224, USA.
出版信息
Mol Genet Metab. 2013 May;109(1):21-7. doi: 10.1016/j.ymgme.2013.02.002. Epub 2013 Feb 13.
BACKGROUND
Very-long-chain acyl-CoA dehydrogenase (VLCAD) deficiency (VLCADD) is diagnosed in the US through newborn screening (NBS). NBS often unequivocally identifies affected individuals, but a growing number of variant patterns can represent mild disease or heterozygous carriers.
AIMS
To evaluate the validity of standard diagnostic procedures for VLCADD by using functional in vitro tools.
METHODS
We retrospectively investigated 13 patient samples referred to our laboratory because of a suspicion of VLCADD but with some uncertainty to the diagnosis. All 13 patients were suspected of having VLCADD either because of abnormal NBS or suggestive clinical findings. ACADVL genomic DNA sequencing data were available for twelve of them. Ten of the patients had an abnormal NBS suggestive of VLCADD, with three samples showing equivocal results. Three exhibited suggestive clinical findings and blood acylcarnitine profile (two of them had a normal NBS and the third one was unscreened). Assay of VLCAD activity and immunoblotting or immunohistologic staining for VLCAD were performed on fibroblasts. Prokaryotic mutagenesis and expression studies were performed for nine uncharacterized ACADVL missense mutations.
RESULTS
VLCAD activity was abnormal in fibroblast cells from 9 patients (8 identified through abnormal NBS, 1 through clinical symptoms). For these 9 patients, immunoblotting/staining showed the variable presence of VLCAD; all but one had two mutated alleles. Two patients with equivocal NBS results (and a heterozygous genotype) and the two patients with normal NBS exhibited normal VLCAD activity and normal VLCAD protein on immunoblotting/staining thus ruling out VLCAD deficiency. Nine pathogenic missense mutations were characterized with prokaryotic expression studies and showed a decrease in enzyme activity and variable stability of VLCAD antigen.
CONCLUSIONS
These results emphasize the importance of functional investigation of abnormal NBS or clinical testing suggestive but not diagnostic of VLCADD. A larger prospective study is necessary to better define the clinical and metabolic ramifications of the defects identified in such patients.
背景
长链酰基辅酶 A 脱氢酶(VLCAD)缺乏症(VLCADD)在美国通过新生儿筛查(NBS)进行诊断。NBS 通常能明确识别出受影响的个体,但越来越多的变异模式可能代表轻度疾病或杂合子携带者。
目的
使用功能体外工具评估 VLCADD 标准诊断程序的有效性。
方法
我们回顾性调查了 13 例因疑似 VLCADD 但诊断存在一定不确定性而送到我们实验室的患者样本。这 13 名患者均因异常 NBS 或提示临床发现而被怀疑患有 VLCADD。其中 12 名患者的 ACADVL 基因组 DNA 测序数据可用。其中 10 例患者的 NBS 异常提示 VLCADD,其中 3 例结果不确定。3 例患者出现提示性临床发现和血液酰基肉碱谱(其中 2 例 NBS 正常,1 例未筛查)。对成纤维细胞进行 VLCAD 活性测定、免疫印迹或 VLCAD 免疫组化染色。对 9 个未鉴定的 ACADVL 错义突变进行了原核突变和表达研究。
结果
9 例患者的成纤维细胞 VLCAD 活性异常(8 例通过异常 NBS 确定,1 例通过临床症状确定)。对于这 9 名患者,免疫印迹/染色显示 VLCAD 的存在存在差异;除 1 例外,所有患者均有两个突变等位基因。2 例 NBS 结果不确定(且杂合基因型)和 2 例 NBS 正常的患者在免疫印迹/染色中显示正常的 VLCAD 活性和正常的 VLCAD 蛋白,因此排除了 VLCAD 缺乏症。9 个致病性错义突变通过原核表达研究进行了鉴定,结果表明酶活性降低和 VLCAD 抗原的稳定性不同。
结论
这些结果强调了对异常 NBS 或临床检测进行功能研究的重要性,这些检测提示但不能诊断 VLCADD。需要进行更大的前瞻性研究,以更好地定义此类患者中发现的缺陷的临床和代谢后果。
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