Proteolipid protein 1 gene sequencing of hereditary spastic paraplegia

PCR amplification and sequencing of whole blood DNA from an individual with hereditary spastic paraplegia, as well as family members, revealed a fragment of proteolipid protein 1 （PLP1） gene exon 1, which excluded the possibility of isomer 1 expression for this family. The fragment sequence of exon 3 and exon 5 was consistent with the proteolipid protein 1 sequence at NCBI. In the proband samples, a PLP1 point mutation in exon 4 was detected at the basic group of position 844, T→C, phenylalanine→leucine. In proband samples from a male cousin, the basic group at position 844 was C, but gene sequencing signals revealed mixed signals of T and C, indicating possible mutation at this locus. Results demonstrated that changes in PLP1 exon 4 amino acids were associated with onset of hereditary spastic paraplegia.

Research progress of hsa-miR-495-3p and proteolipid protein 1 involvement in the pathogenesis of schizophrenia

Schizophrenia(SCZ)is a serious mental illness whose etiology and pathogenesis are not yet clear.The level of miRNA may be a crucial factor in the occurrence and development of SCZ.This study found that miR-495 may regulate the susceptibility gene of SCZ and that proteolipid protein 1(PLP1)as a risk gene for schizophrenia may be involved in its pathogenesis.In this article we review the research progress related to hsa-miR-495-3p(miR-495),PLP1,and schizophrenia.

Research progress on the mechanism of N6-methylade-nosine methylation modification and proteolipid protein 1 gene in schizophrenia

Schizophrenia (SCZ) is a serious mental illness with unknown etiology, high recurrence rate and high disability rate, which has caused a great burden to individuals and society. There is no clear etiology and pathogenesis. Methylation of N6-methyladenosine (m6A) can regulate the nervous and mental system, and affect the function of the nervous system. Proteolipid protein 1 (PLP1) is a risk gene for schizophrenia. In this study we review the research progress on the pathogenesis of schizophrenia, m6A methylation, and PLP1 gene.

Characterization of proteolipid protein-peptide-specific CD_4^+ T cell of experimental allergic encephalomyelitis in Biozzi AB/H mice

To detect the function of proteolipid protein (PLP) peptide (residues 56-70) sp ecific CD 4 + T cells in experimental allergic encephalomyelitis (EAE) in Bioz zi AB/H mice (H 2A g7 ) Methods Biozzi AB/H mice were immunized by synthetic PLP 56 70 peptide (DYEYLINVIH AFQYV) which was emulsified by sonication with complete Freund’s adjuvant, a EAE model proven histologically and clinically Murine splenocytes and spinal cord infiltrated (SCI) T cells were stimulated by PLP 56 70 , then the CD 4 + T cells were isolated by Dynabeads, and confirmed by staining with anti CD 4 antibody Finally, the IL2 bioassay and IFN γ/IL4 ELISA were done to detect T cell proliferation and cytokine secretion after PLP 56 70 stimulation Results The histology of murine spinal cord showed a great number of lymphocytes infiltr ated the spinal cord; the clinical signs showed high scores (4 3) on the peak, as well as a good EAE model After being isolated by Dynabea ds , CD 4 + T cells showed high purification (>99%) by staining with anti CD 4 antibody IL2 bioassay showed that those T cells were PLP 56 70 specific T cells ELISA showed that those T cells had high IFN γ/IL4 ratio , indicating that they are T helper 1 (Th1) cells Conclusions PLP 56 70 specific splenocytes and SCI CD 4 + T cells in EAE from Bioz zi AB/H mice were detected and showed that both of them were P LP 56 70 specific Th1 cells It is beneficial to understand what kind o f role these T cells play in the development of

神经干细胞移植对脊髓损伤后PLP基因表达的影响

目的: 研究神经干细胞(NSCs) 移植对大鼠脊髓损伤(SCI) 后髓鞘蛋白前脂蛋白(PLP) 基因表达的影响, 探讨神经干细胞移植促进大鼠SCI后髓鞘再生的机制。方法:NSCs由5-溴-2脱氧尿嘧啶核苷标记法(Brdu) 标记。实验分为3组: NSCs移植组(A组)、DMEM填充组(B组)、正常对照组(C组)。大鼠SCI后第7d移植NSCs, 应用免疫组化和RT-PCR法观察NSCs移植后是否存活, 以及大鼠脊髓损伤区PLP基因表达的动态变化。结果: NSCs移植后在受体脊髓内存活, NSCs移植组较单纯损伤组明显促进了PLP基因在分子和蛋白水平的表达。结论: NSCs移植后可存活并促进PLP基因的表达, 是促进脊髓损伤后髓鞘再生的机制之一。

蛋白脂蛋白在两型星形胶质细胞和少突胶质细胞中的表达

目的:探讨蛋白脂蛋白(PLP)在分化成熟的两型星形胶质细胞和少突胶质细胞中的表达。方法:用激光共聚焦双重免疫荧光标记技术检测PLP在分化成熟的两型星形胶质细胞和少突胶质细胞中的表达情况。结果:在O-2A谱系来源的成熟2型星形胶质细胞和少突胶质细胞中PLP抗体标记为阳性,而在T1A谱系来源的成熟1型星形胶质细胞中则未检测到PLP的表达,从而在蛋白质水平验证本室研究两型星形胶质细胞基因表达谱差异基因芯片结果中PLP mRNA在T2A中高表达,而在T1A中低表达的现象。结论:PLP等脂代谢相关基因可能在O-2A谱系发生和分化过程中起重要作用,O-2A谱系与神经髓鞘发生以及脑内脂质代谢内在机制密切相关。

髓鞘蛋白脂质蛋白多肽_(139-151)诱发实验性自身免疫性脑脊髓炎小鼠模型

目的 用髓鞘蛋白脂质蛋白多肽 (PLP) 1 39- 1 5 1 诱发实验性自身免疫性脑脊髓炎 (EAE)小鼠模型。方法 应用 PLP1 39- 1 5 1 抗原加完全福 (氏 )佐剂免疫 SWXJ小鼠。结果 免疫 1 4～ 2 0 d后小鼠即发病 ,发病率为 80 % ,而且多数呈缓解 -复发型。病理学证实发病小鼠脑和脊髓内具有典型的脱髓鞘改变和炎性细胞浸润。结论 以PLP1 39- 1 5 1 为抗原免疫 SWXJ小鼠诱发 EAE,具有模型稳定、发病率高和缓解 -复发的特点 。

PLP不同肽段诱导EAE模型的对比研究

目的建立不仅与多发性硬化(multiplesclerosis,MS)临床表现、病理特征接近而且病程相似的较为理想的复发缓解型实验性自身免疫性脑脊髓炎(experimentalautoimmuneencephalomyelitis,EAE)模型。方法应用髓鞘蛋白脂质蛋白(proteolipidprotein,PLP)多肽的两种免疫优势表位肽段PLP139151和PLP178191免疫雌性SJL/J小鼠,制作复发缓解型EAE(relapseremittingexperimentalautoimmuneencephalomyelitis,RREAE)模型,观察其体重及神经功能评分的变化,应用HE、Luxolfastblue髓鞘染色等方法观察模型的组织形态学改变。结果两种PLP肽段免疫的小鼠发病均具有缓解复发的特点,出现明显的神经系统体征;小鼠发病时脑和脊髓组织显示明显的血管鞘形成、卫星现象和炎性细胞浸润以及脱髓鞘改变。结论PLP两种肽段均可诱发RREAE模型,这与临床MS的缓解复发病程更相似,更能表现MS的临床特点,是研究MS的较为理想的动物模型。

脊髓损伤大鼠骨髓基质细胞移植后BDNFmRNA、GDNFmRNA及PLPmRNA的表达

目的:研究骨髓基质细胞(BMSCs)移植对大鼠脊髓损伤(SCI)后脑源性神经营养因子(BDNF)、胶质细胞源性神经营养因子(GDNF)、髓鞘前脂蛋白(PLP)基因表达的影响,探讨BMSCs促进SCI修复的机制。方法:Wistar大鼠42只,随机分为移植组(A组)和对照组(B组)各18只,制成SCI模型,将培养的BMSCs注入移植组损伤的脊髓内;另6只为假手术组(C组)。结果:术后24和72h、7d,RT-PCR半定量分析显示A、B组BDNFmRNA、GDNFmRNA和PLPmRNA表达在24及72h、7d时均明显高于C组(P<0.01),与B组比较,A组升高更显著(P<0.05)。结论:BM-SCs移植可通过促进神经营养因子的表达和轴突髓鞘化等机制促进SCI修复。

Proteolipidprotein 1 gene mutation in nine patients with Pelizaeus-Merzbacher disease

Background Pelizaeus-Merzbacher disease （PMD） is a rare X-linked recessive disorder with symptoms including nystagmus, impaired motor development, ataxia, and progressive spasticity. The proteolipidprotein 1 （PLP1） gene is the only pathogenic gene of PMD. Duplication of the PLP1 gene is the most frequent gene defect, accounting for 50%-70% of PMD cases, whereas point mutations in the coding sequence or the splice sites account for 10%-25% of PMD cases. This study aimed to identify PLP1 mutations in nine unrelated Chinese patients （P1-9） with PMD, and 14 subjects from the family of patient 2 were also described. Methods Genomic DNA was extracted from peripheral multiplex ligation-dependent probe amplification （MLPA）. AI amplified and analyzed using direct DNA sequencing. blood samples. Gene dosage was determined using the 7 exons and exon-intron boundaries of the PLP1 gene were Results Of these nine patients, there were four transitional, four classical, and one connatal PMD according to their clinical and radiological presentations. PLP1 duplications were identified in patients 1-7 with PMD. Their mothers were PLPI duplications carriers as well. Both duplication carriers and normal genotypes of PLP1 were identified in the family members of patient 2. A c.517C〉T （p. P173S） hemizygous missense mutation in exon 4 was found in patient 8 with PMD, and his mother was shown to be a heterozygote of this mutation. Conclusions We identified seven genomic duplications and one missense mutation （p. P173S） of the PLP1 gene in eight Chinese patients with PMD. This is the report about PLP1 mutations in PMD patients from the mainland of China.

老化大鼠髓鞘蛋白脂蛋白表达变化及意义

目的观察老化大鼠髓鞘蛋白PLP的改变、髓鞘结构、中枢传导功能变化及其关系。方法采用免疫组化方法检测大鼠老化时髓鞘蛋白PLP表达变化,透射电镜观察脑白质区域的超微结构变化,电生理方法记录中枢神经传导功能。结果PLP免疫组化:2组于纹状体、胼胝体、前联合、皮层下区均可见阳性染色。但老年组大鼠各部位PLP表达量明显减少,其积分光密度值明显增大(P<0.01)。白质区超微结构变化:老年大鼠轴突直径增加,轴突内含有巨大线粒体,轴突周围间隙扩大。髓鞘致密层分离,部分板层结构排列紊乱、破坏。中枢传导功能:2组间存在显著差别,老年大鼠中枢传导潜伏时较青年组显著延长(P<0.01)。结论髓鞘蛋白PLP表达减少,与髓鞘形态结构改变有关,髓鞘及轴突超微结构存在明显变化,是白质功能减退的重要原因,这种变化可能与大鼠老化时中枢神经传导功能降低有关。

神经髓鞘及脱脂神经髓鞘诱导MS-TCL增殖反应比较

目的 比较神经髓鞘和脱脂神经髓鞘诱导多发性硬化(MS)T淋巴细胞系(TCL)对11种神经髓鞘成份的增殖反应。方法 以2种人神经髓鞘在体外二次致敏,诱导MS-TCL和正常人TCL,用MBP、PLP及其合成多肽等抗原检测PTL的增殖反应。结果 与非脱脂TCL相比,脱脂髓鞘使MS组的免疫反应性显著改变。尤其对PLP6种多肽反应性的改变有统计学差异,总平均阳性孔比较P<0.001(3.41±4.83 vs 5.49±5.31)。结论 髓鞘脱脂使MS组增殖反应显著增加,二组的差别更明显。提示在髓鞘脱脂方面MS和正常人反应的异质性,此点对理解MS的病理机制可能很重要。

脱脂神经髓鞘诱导多发性硬化T淋巴细胞系增殖反应分析

目的 揭示中枢神经髓鞘脱脂过程在多发性硬化 (MS)发生发展中的作用。方法 以人脱脂神经髓鞘二次致敏诱导MS患者T淋巴细胞系 (MS TCL) ,用髓鞘碱性蛋白 (MBP)、蛋白脂蛋白 (PLP)及其合成多肽等抗原检测TCL的增殖反应。结果 MS组对 11种抗原均有较强反应 ,对 7种抗原的反应性与对照组间有差异 (P <0 0 5 ) ,两组总和平均阳性孔比较P <0 0 0 1(5 49± 5 31与3 10± 3 17比较 )。结论 PLP和MBP与MS发病有关 ;M87 10 6、P95 117、P40 6 0、P185 2 0 6等序列可能是致病抗原决定簇 ;MS病人体内可能有神经髓鞘异常脱脂。

实验性自身免疫性脑脊髓炎中γδT细胞的变化及血吸虫卵抗原干预对其的影响

目的:研究髓鞘蛋白脂质蛋白多肽178-191(PLP178-191)免疫后小鼠体内γδ T细胞比例的变化以及日本血吸虫虫卵抗原(SEA)干预对其的影响。方法:用流式细胞仪检测技术分别观察对照组、PLP178-191免疫组、SEA干预组小鼠肠上皮内CD3+细胞中γδ T细胞百分比的变化。结果:对照组肠上皮内淋巴细胞CD3+细胞中γδ T细胞百分比为(22.95±7.26)%,PLP178-191免疫组γδ T细胞比例明显升高(P<0.01),SEA干预组则较PLP178-191免疫组有所下降(P<0.01)。结论:γδ T细胞与实验性自身免疫性脑脊髓炎(EAE)发病可能有着密切关系。EAE的干预能使γδ T细胞升高幅度有一定程度的降低,这可能是SEA用于EAE治疗研究的机制之一。

兄弟两人同患佩梅病临床及基因分析

目的探讨佩梅病的临床、影像及遗传学特征。方法回顾分析及随访1个核心家系中兄弟两人同患佩梅病的临床资料。结果先证者男性,7岁,弟弟5岁,均表现为自幼运动发育迟缓,不能独站、独走,而智力发育基本不受影响。T2加权像头颅磁共振成像表现为脑白质弥漫性高信号。先证者及弟弟均存在蛋白脂蛋白1(PLP 1)基因c.259 delC半合子变异;母亲为携带者。兄弟两人均确诊为中间型佩梅病。随访3年,运动功能异常加重,先证者仅能短暂扶站,四肢肌力Ⅲ级;先证者弟弟足踝变形,明显足内翻,无法扶站;智力均无明显倒退。结论发现国内未见报道的PLP1基因c.259 delC半合子变异所致佩梅病。

佩利措伊斯-梅茨巴赫病临床及遗传学特征分析

目的探讨佩利措伊斯-梅茨巴赫病(PMD)的临床及分子遗传学特征。方法回归性分析2015年6月至2020年10月郑州大学第三附属医院确诊的12个家系共14例PMD患儿的临床表现和基因突变特点。结果14例均为男性,就诊年龄5 d至10岁,起病年龄1 d至7个月。首发症状表现为眼球震颤9例,大运动发育迟缓3例,呻吟样呼吸、哭声弱1例,异常姿势2例。临床表现:14例均存在发育迟缓,其中10例以运动发育迟缓更为明显;肌张力低下10例,肌张力增高3例;12例存在眼球震颤。临床分型经典型8例,先天型2例,中间型4例。14例患儿头颅磁共振成像(MRI)均表现为脑白质髓鞘化障碍,脑干听觉诱发电位检测异常7例。14例先证者中,7例蛋白脂蛋白1(PLP1)基因为2~8号外显子重复变异;1例为X染色体Xq22.2处重复0.33Mb区域,覆盖了PLP1基因100%的区域;1例c.83G>A变异,1例c.226G>C变异,2例c.259delC变异,2例c.157dupA变异。12例先证者为遗传性突变,均为母源遗传,母亲为无临床症状的携带者。c.83G>A、c.226G>C、c.259delC、c.157dupA均为国际上未报道的新突变。结论PMD的首发症状以眼球震颤最为常见;发育迟缓、肌张力异常、眼球震颤为其最常见的临床症状;头颅MRI提示脑白质髓鞘化障碍。PLP1基因突变中重复变异最多,其次为点突变,c.83G>A、c.226G>C、c.259delC、c.157dupA变异为尚未报道的新突变。

多发性硬化症髓鞘素组分特异性抗体分泌细胞

本文用酶联免疫班点法(Elispot)检测了23例临床确诊多发性硬化症(MS)和12例无菌性脑膜炎(AM)患者外周血(PB)和脑脊液(CSF)中髓鞘素碱性蛋白(MBP)、髓鞘素结合糖蛋白(MAG)和含脂质蛋白(PLP)特异性IgG抗体分泌细胞。两组患者CSF中该3种抗体分泌细胞均呈明显增多趋势,MS组尤著,但两组PB中该类细胞数均很少。指示对髓鞘素组分的B细胞免疫应答主要局限于与中枢神经系统(CNS)近邻的CSF中,可能是鞘内合成IgG抗体的重要来源。

遗传性痉挛性截瘫2型一家系PLP1基因突变分析

目的分析并确定一个遗传性痉挛性截瘫2型(spastic paraplegia 2,SPG2)家系蛋白脂蛋白1(proteolipid protein 1,PLP1)基因突变与遗传学特征。方法收集先证者及其家系成员临床资料,采用聚合酶链反应和DNA直接测序方法进行PLP1基因突变检测,确定基因突变位点,分析基因型与表型的关系。结果本家系先证者临床符合SPG2诊断。测序结果显示先证者PLP1基因第3外显子c.388C>T(p.His130Tyr)半合子改变,先证者之母为本位点的杂合改变。结论本家系SPG2先证者为PLP1基因半合子突变致病,遗传自表型正常携带者的母亲。本研究明确了本家系PLP1基因突变与遗传特征,为准确的遗传咨询和进一步的产前诊断打下了基础。

幼年和成年大鼠视皮层蛋白脂质蛋白质的基因表达

目的观察蛋白脂质蛋白质(proteolipid protein,PLP)基因在幼年和成年大鼠视皮层中的表达水平,探讨其在视觉可塑性关键期中的作用。方法采用半定量RT-PCR方法,分析处于视觉可塑性关键期内的幼年大鼠和处于视觉可塑性关键期后的成年大鼠视皮层中PLP基因的表达水平。结果幼年大鼠和成年大鼠视皮层间PLP mRNA表达量有显著性差异,PLP mRNA在幼年大鼠视皮层中表达水平显著高于成年大鼠。结论PLP基因在视觉可塑性关键期内的幼年大鼠视皮层中呈高水平表达,证实了PLP基因是视觉可塑性相关基因,参与了视觉可塑性关键期的调控。

PLP2在心肌重构中的动态表达变化

目的探讨PLP2蛋白在心肌重构心脏组织和心脏各类细胞中的表达改变。方法用冠状动脉左前降支结扎术建立小鼠心肌梗死后的心脏重构模型、异丙肾上腺素(ISO)皮下注射2周建立小鼠急性心脏损伤模型;胸主动脉结扎术(aortic banding,AB)建立小鼠心肌肥厚的模型。苯肾上腺素诱(PE)导心肌细胞肥大模型;转化生长因子(TGF)β刺激心肌成纤维细胞激活。采用RT-PCR检测上述各种心脏重构模型中PLP2转录水平的改变。结果 PLP2在小鼠心肌梗死(miocardial infarction,MI)术后2周表达明显增高(P<0.05);在ISO诱导的急性心脏损伤后2周表达增高(P<0.05);在AB术后1周表达开始增高(P<0.05),在AB术后2周达到高峰(P<0.05),持续到AB术后8周(P<0.05)。PLP2在PE诱导的心肌细胞肥大模型中表达增高;在TGFβ刺激的成纤维细胞中表达明显增高。结论 PLP2的表达在不同模型的心脏重构中均发生明显改变,且呈现动态变化,提示其可能参与心脏重构的发生、发展。