家族性多发性结肠息肉家族成员的细胞遗传学研究

目的 揭示家族性多发性结肠息肉以及癌变的机理 ,为癌前监控和早期发现提供可靠的科学依据。方法 用RPMI 16 4 0和Tc 199培养基 ,采用微量全血培养法 ,在正常叶酸和低叶酸两种培养条件下 ,对 3个家族性多发性结肠息肉家系中的 6 1名成员的外周血淋巴细胞进行了较全面的染色体分析。结果 发现在正常叶酸和低叶酸培养条件下 ,绝大多数家族性多发性结肠息肉患者外周血染色体畸变率明显升高 ,正常叶酸组FPC患者为 6 .95 %,低叶酸组FPC患者为 10 .5 %。患者中出现的脆性部位频率较高的有 3p14、1p2 2和1p32等。 结论 家族性多发性结肠息肉患者染色体脆性部位表达率明显高于正常对照组 ,且染色体脆性部位与癌基因、癌断点具有一定的相关性。

家族性慢性良性天疱疮一家系ATP2C1基因突变检测

目的研究家族性慢性良性天疱疮一家系的ATP2C1基因突变情况。方法采用聚合酶链反应(PCR)及直接测序的方法对家系中4例患者ATP2C1基因进行突变检测,以家系中3例健康者和100例无血缘关系的正常人作对照。结果该家系4例患者ATP2C1基因的7号外显子第457位碱基胞嘧啶C被胸腺嘧啶T替代,导致第153位的精氨酸被终止密码子取代(R153X),家系中健康对照及无血缘关系的正常人均未发现该突变。结论无义突变c.457C>T(p.R153X)是导致该家系发病的主要原因。

家族性玻璃体淀粉样变性患者甲状腺激素结合蛋白基因突变研究

玻璃体淀粉样变性是一种少见的眼部局限性遗传性淀粉样变性，国内迄今报道不足20例。患者常伴家族史，其遗传方式均为常染色体显性遗传。目前已知造成遗传样淀粉样变性基因突变的物质有7种。研究最多、并与眼部淀粉样变性特别是与玻璃体淀粉样变性密切相关的基因为甲状腺激素结合蛋白（TTR），但其突变位点多样化，

家族性玻璃体淀粉样变性甲状腺激素结合蛋白Gly83Arg突变一家系

家族性玻璃体淀粉样变性（FTA）属常染色体显性遗传性疾病。因淀粉样物质在玻璃体沉积致病。研究最多并与眼部淀粉样变性特别是与玻璃体淀粉样变性密切相关的基因为甲状腺激素结合蛋白（TTR）；目前已知和淀粉样变性相关的TTR基因突变有100多种。

无家族史及系统表现的双眼玻璃体淀粉样变性一例

患者男,55岁。因左眼无痛性视力逐渐下降2个月于2016年2月来北京大学第三医院眼科就诊。既往身体健康,否认系统病史及家族遗传病史。眼部检查:右眼视力1.0,左眼视力数指。双眼眼压均为12 mmHg(1 mmHg=0.133 kPa)。右眼眼前后节均未见异常。左眼眼前节未见异常;玻璃体灰白色混浊,眼底模糊。B型超声检查,左眼玻璃体团状中等回声,后脱离。初步诊断:左眼玻璃体陈旧积血(原因待查)。行左眼玻璃体切割手术,手术中见玻璃体呈白色棉絮状,眼底未见异常。手术后1个月复查,左眼视力1.0。2017年8月,患者以右眼视力逐渐下降2个月及左眼视物模糊1个月再次就诊,否认其他任何不适。全身查体及实验室检查无阳性发现。眼部检查:右眼、左眼BCVA分别为0.1、0.8。右眼、左眼眼压分别为15、12 mmHg。双眼眼前节未见异常。右眼玻璃体白色絮状混浊,晶状体后玻璃体呈白色斑点状。

家族性玻璃体淀粉样变性甲状腺激素结合蛋白基因突变及表达研究

目的 观察家族性玻璃体淀粉样变性（FTA）一家系甲状腺激素结合蛋白（TTR）基因突变位点及其mRNA、蛋白表达变化.方法 来自同一家系的家族性玻璃体淀粉样变性患者7例（发病组）、家系中未发病成员19名（未发病组）以及与该家系来自同一地区的正常健康者9名（对照组）纳入研究.采集3组受检者外周静脉血,提取DNA,采用逆转录聚合酶链反应（PCR）扩增TTR基因外显子1～4,进行测序.实时荧光定量PCR检测受检者血细胞中TTR mRNA的表达.蛋白免疫印迹法检测受检者血清中TTR蛋白表达.结果 发病组7例、未发病组3名受检者TTR外显子3的107位碱基出现杂合突变,由G变为C,出现套峰;即第83氨基酸的密码子发生碱基突变,由GGC突变成CGC,甘氨酸突变为精氨酸（Gly83Arg）,其氨基酸的极性由中性转变为碱性.其他受检者未发现该位点基因突变.发病组患者TTRmRNA表达均较未发病组、对照组低,差异有统计学意义（P=0.032、0.001）;未发病组受检者血细胞中TTR mRNA表达较对照组低,差异有统计学意义（P=0.001）.发病组患者血清中TTR蛋白表达均较未发病组、对照组低,差异有统计学意义（P=0.035、0.038）;未发病组与对照组受检者血清中TTR蛋白表达比较,差异无统计学意义（P=0.491）.结论 该家系7例患者、3名未发病家系成员TTR基因第3外显子发生杂合突变,即Gly83Arg.发病患者TTR mRNA及蛋白表达较未发病家系成员及正常者降低.

Migraine as a sex-conditioned inherited disorder: evidences from China and the world

Migraine is a complex and heterogeneous disorder. Although several genetic models has been proposed including autosomal-dominant/autosomal recessive, sex-linked, sex-limited, mitochondrial, and multi-gene, none of these models can well-explain the transmission of the disease. We hypothesied that migraine is a sex-conditioned inherited disorder （autosomal dominant in females and autosomal recessive in males）. This hypothesis is supported by the evidence such as the locations of genes associated with familial hemiplegic migraine, possibly ＂typical＂ migraine as well （dominantly on chromosome 19p, lq, and 2q）, male：female ratio of prevalence （1：2-1：4）, the mostly youth-onset, the provocation by the contraceptives, the induction by menstruation, and the self-limitation after menopause. Female sex-hormones appear to be the key contributor to a higher prevalence of migraine in female. Socio-environmental factors may also play an important role.

Germline MLH1 and MSH2 mutational spectrum including frequent large genomic aberrations in Hungarian hereditary non-polyposis colorectal cancer families:Implications for genetic testing

AIM: To analyze the prevalence of germline MLH1 and MSH2 gene mutations and evaluate the clinical characteristics of Hungarian hereditary non-polyposis colorectal cancer (HNPCC) families. METHODS: Thirty-six kindreds were tested for mutations using conformation sensitive gel electrophoreses, direct sequencing and also screening for genomic rearrangements applying multiplex ligation-dependent probe amplifi cation (MLPA). RESULTS: Eighteen germline mutations (50%) were identifi ed, 9 in MLH1 and 9 in MSH2. Sixteen of these sequence alterations were considered pathogenic, the remaining two were non-conservative missense alterations occurring at highly conserved functional motifs. The majority of the defi nite pathogenic mutations (81%, 13/16) were found in families fulfilling the stringent Amsterdam Ⅰ/Ⅱ criteria, including three rearrangements revealed by MLPA (two in MSH2 and one in MLH1). However, in three out of sixteen HNPCC-suspected families (19%), a disease-causing alteration could be revealed. Furthermore, nine mutations described here are novel, and none of the sequence changes were found in more than one family.CONCLUSION: Our study describes for the f irst time the prevalence and spectrum of germline mismatch repair gene mutations in Hungarian HNPCC and suspected-HNPCC families. The results presented here suggest that clinical selection criteria should be relaxed and detection of genomic rearrangements should be included in genetic screening in this population.

Familial Wolff-Parkinson-White syndrome is linked to the loci on chromosome 7q3

OBJECTIVE: Wolff-Parkinson-White syndrome (WPW) is considered to be an autosomal dominant hereditary disease, but the gene is not identified. The objective of this study was to localize the genetic loci of Wolff-Parkinson-White syndrome. METHODS: Linkage analysis between the disease of Wolff-Parkinson-White syndrome and 3 STR (short tandem repeats) markers on 7q3 (D7S505, D7S688, and D7S483) was tested in 3 kindreds of the Wolff-Parkinson-White syndrome (101 numbers in total) by genotyping. RESULTS: Wolff-Parkinson-White syndrome was linked to the loci above. The maximum two-point Lod score detected at D7S505 was 6.4 at a recombination fraction (theta) of 0.1; the Lod score of D7S688, D7S483 was 5.3 vs 2.5. CONCLUSION: The gene of Wolff-Parkinson-White syndrome is located at 7q3.