Proline with or without Hydroxyproline Influences Collagen Concentration and Regulates Prolyl 4-Hydroxylase α(I) Gene Expression in Juvenile Turbot(Scophthalmus maximus L.)

This study was conducted to investigate the effect of dietary proline(Pro), and Pro and hydroxyproline(Hyp) in combination on the growth performance, total Hyp and collagen concentrations of tissues, and prolyl 4-hydroxylase α(I)(P4H α(I)) gene expression in juvenile turbot feeding high plant protein diets. A diet containing 50% crude protein and 12% crude lipid was formulated as the basal and control, on which other two protein and lipid contents identical experimental diets were formulated by supplementing the basal with either 0.75% Pro(Pro-0.75) or 0.75% Pro and 0.75% Hyp(Pro+Hyp). Four groups of fish in indoor seawater recirculating systems, 35 individuals each, were fed twice a day to apparent satiation for 10 weeks. The results showed that dietary Pro and Hyp supplementation had no significant effect on growth performance and feed utilization of juvenile turbot(P > 0.05). Total Hyp and collagen concentrations in muscle were significantly increased when dietary Pro and Hyp increased(P < 0.05), and fish fed diet Pro+Hyp showed significantly higher free Hyp content in plasma than those fed other diets(P < 0.05). The expression of P4 H α(I) gene in liver and muscle was significantly up regulated in fish fed diet Pro-0.75 in comparison with control(P < 0.05); however the gene was significantly down regulated in fish fed diet Pro+Hyp in muscle in comparison with fish fed diet Pro-0.75(P < 0.05). It can be concluded that supplement of crystal L-Pro and L-Hyp to high plant protein diets did not show positive effects on growth performance of juvenile turbot, but enhanced total collagen concentrations in muscle.

Prognostic value of hypoxia-inducible factor-1 alpha and prolyl 4-hydroxylase beta polypeptide overexpression in gastric cancer

AIM To investigate the relationship between hypoxia-inducible factor-1α(HIF-1α), prolyl 4-hydroxylase beta(P4 HB) expression, and clinicopathologic parameters, as well as the prognostic value of these genes for patients with gastric cancer(Gc).METHODS Hypoxia is a critical factor that shapes the Gc microenvironment. In previous reports, we have demonstrated that P4 HB is a potential target of HIF-1α. In the present study, gene expression profiling interactive analysis(GEPIA) was used to analyze the relationship between P4 HB and hypoxia-associated genes. To this end, 428 Gc tissue samples were used to analyze the expression of HIF-1α and P4 HB via immunohistochemical staining. Patient samples were classified as having weak-expression or over-expression both in terms of HIF-1α and P4 HB. Correlations between biomarkers and clinicopathological factors were analyzed to predict survival. RESULTS P4 HB demonstrated a positive correlation with hypoxiaassociated genes(P < 0.05). HIF-1α and P4 HB overexpression have a significant correlation with TNM staging(χ2 = 23.32, P = 0.00; χ2 = 65.64, P = 0.00) and peritoneum cavity metastasis(χ2 = 12.67, P = 0.00; χ2 = 39.29, P = 0.00). In univariate analysis, patients with a high HIF-1α expression trend had a shorter disease-free survival(DFS: 44.80 mo vs 22.06 mo) and overall survival(OS: 49.58 mo vs 39.92 mo). P4 HB overexpression reflected similar results: patients with over-expression of P4 HB had a shorter survival time than those with weak-expression(DFS: 48.03 mo vs 29.64 mo, OS: 52.48 mo vs 36.87 mo). Furthermore, HIF-1α is also a clinicopathological predictor of dismal prognosis according to multivariate analysis(DFS, 95%c I: 0.52-0.88, P < 0.00; OS, 95%c I: 0.50-0.85, P < 0.00). However, P4 HB was meaningful in DFS(95%c I: 0.58-1.00, P < 0.05) but not in OS(95%c I: 0.72-1.23, P > 0.05).CONCLUSION Overexpression of HIF-1α and P4 HB is associated with poor prognosis in patients with Gc. Thus, these genes may be potential prognostic biomarker candidates in GC.

Isolation and Expression Analysis of Two Genes Encoding Cinnamate 4-Hydroxylase from Cotton(Gossypium hirsutum)

Two genes （GhC4H1 and GhC4H2） that encode putative cotton cinnamate 4-hydroxylases that catalyze the second step in the phenylpropanoid pathway were isolated from developing cotton fibers. GhC4H1 and GhC4H2 each contain open reading frames of 1 518 base pairs （bp） in length and both encode proteins consisting of 505 amino acid residues. They are 90.89% identical to each other at the amino acid sequence level and belong to class I of plant C4Hs. GhC4H1 and GhC4H2 genomic DNA are 2 247 and 2 161 bp long, respectively, and contain two introns located at conserved positions relative to the coding sequence. GhC4HI and GhC4H2 promoters were isolated and found to contain many cis-elements （boxes P, L and AC-1 element） previously identified in the promoters of other phenylpropanoid pathway genes. Histochemical staining showed GUS expression driven by the GhC4H1 and GhC4H2 promoters in ovules and fibers tissues. GhC4H1 and GhC4H2 were also widely expressed in other cotton tissues. GhC4H2 expression reached its highest level during the elongation stage of fiber development, whereas GhC4H1 expression increased during the secondary wall development period in cotton fibers. Our results contribute to a better understanding of the biochemical role of GhC4H1 and GhC4H2 in cotton fiber development.

脯氨酰-4-羟化酶亚基α-2通过肌醇需要酶1α介导的UPR信号通路调控肝癌细胞凋亡并预测早期肝细胞癌的不良预后

肝细胞癌(hepatocellular carcinoma,HCC)严重危害着人类健康。尽管大量研究表明,在HCC早期进行手术切除可提高患者的生存率,但其高复发率仍然阻碍着治疗进程。本研究分析蛋白质组学数据发现。脯氨酰-4-羟化酶亚基α-2(prolyl 4-hydroxylase subunit α-2,P4HA2)在早期HCC组织中高表达,Kaplan-Meier曲线、Cox比例风险回归模型(cox regression model)证明,P4HA2高表达的早期肝癌患者预后较差,且P4HA2可作为患者预后的独立预测因子。通过敲低或过表达实验发现,P4HA2明显促进肿瘤细胞的增殖、迁移等恶性生物学行为。敲低P4HA2激活了由肌醇需要酶1α(inositol-requiring enzyme 1α,IRE1α)介导的促凋亡非折叠蛋白反应(unfolded protein response,UPR)。以上结果表明,P4HA2可能通过调节内质网稳态来调控肝癌细胞凋亡,P4HA2有望成为HCC潜在的治疗靶点。

脯氨酰4-羟化酶α亚单位3在胃癌中的表达及临床意义

目的 探讨脯氨酰4-羟化酶α亚单位3(P4HA3)在胃癌中的表达及临床意义。方法 通过UALCAN数据库及基因表达综合(GEO)数据库分析胃癌组织和癌旁正常组织中P4HA3基因表达差异,并进一步分析癌症基因组图谱(TCGA)数据库中不同临床分期、分化程度、年龄和性别胃癌患者P4HA3基因表达差异。以P4HA3基因表达中位值为界,将患者分为P4HA3高表达组和P4HA3低表达组,采用Kaplan-Meier plotter在线数据库比较两组患者的总生存时间、首次进展生存时间和进展后生存时间。收集107例胃癌患者的胃癌组织及癌旁正常组织标本,采用免疫组织化学染色法检测P4HA3蛋白表达情况,并结合临床特征及随访资料进行综合分析。结果 TCGA数据库和GEO数据库中的数据均显示,胃癌组织中P4HA3基因表达水平明显高于癌旁正常组织(P﹤0.01)。TCGA数据库显示,不同年龄、分化程度、临床分期胃癌患者的P4HA3基因表达水平比较,差异均有统计学意义(P﹤0.05)。Kaplan-Meier plotter在线数据库分析发现,P4HA3高表达组患者的中位总生存时间、中位首次进展生存时间、中位进展后生存时间均明显短于P4HA3低表达组,差异均有统计学意义(P﹤0.01)。胃癌组织中P4HA3蛋白阳性表达率高于癌旁正常组织(P﹤0.05)。不同肿瘤直径、分化程度、TNM分期、T分期胃癌患者胃癌组织中P4HA3蛋白表达情况比较,差异均有统计学意义(P﹤0.05);P4HA3阴性表达患者的累积生存率明显高于P4HA3阳性表达患者(P﹤0.01)。结论 P4HA3在胃癌组织中高表达,且与胃癌的发生发展及预后有关,可能成为胃癌的预后评估指标和潜在治疗靶点。

桑树绿枝扦插繁殖过程中ABI4和PIN1基因的表达变化及与生根性能的相关性

脱落酸非敏感型转录因子ABI4、生长素运输载体蛋白PIN1分别通过调控脱落酸和生长素的运输而影响植物不定根的发育与生长。以经生根粉诱导处理和未经诱导处理的桑树绿枝插穗为材料,用实时荧光定量PCR、Western blot技术检测插穗生根发育过程中基部皮层ABI4和PIN1基因的转录与蛋白质表达水平变化。当插穗出现不定根时,ABI4的转录与表达水平急剧下调,PIN1的转录水平急剧上调,而后在新生根伸长期二者均有所回复;生根剂诱导处理插穗后加大了其基部皮层ABI4的转录与表达下调幅度和PIN1的转录上调幅度,且PIN1在新生根伸长期持续高表达。ABI4的转录水平与不同桑品种生根率之间均呈显著的负相关关系(γ=-0.915),与生根数量没有相关性;而PIN1的转录水平与生根率和生根数量均呈显著的正相关关系(γ=0.880,γ=0.982)。农桑14号和强桑1号等是绿枝生根率高的桑品种,其插穗不定根出现时基部皮层ABI4的转录、表达下调幅度和PIN1的转录上调幅度大于大10等生根率低的桑品种,提示易生根品种的插穗在不定根出现时期ABI4的低水平和PIN1的高表达会更利于插穗根原基的形成、分化及新生根的生长。

益气除痰方对缺氧微环境下A549细胞上皮间质转化及P4HB表达的影响

目的研究益气除痰方对缺氧条件下A549细胞上皮间质转化的影响并初步探讨其与脯氨酸4-羟化酶β亚基(P4HB)、波形蛋白(Vimentin)表达的相关性。方法将A549细胞分为3组培养:常氧对照组(常规培养),缺氧模型组(加入CoCl2培养模拟缺氧微环境诱导A549细胞上皮间质转化),益气除痰方含药血清组(在CoCl2培养基础上加入益气除痰方含药血清培养)。相差显微镜下观察3组A549细胞形态的变化;RT-PCR检测3组549细胞P4HB、Vimentin mRNA的表达含量。结果相差显微镜下常规培养的A549细胞呈不典型上皮细胞形态,经CoCl2刺激后,大部分细胞形态明显拉长,呈现明显的间质细胞形态。益气除痰方含药血清组与常氧对照组比较间质细胞形态的细胞增多,较缺氧模型组间质细胞形态的细胞明显减少。缺氧模型组A549细胞P4HB、Vimentin mRNA的表达量较常氧对照组明显上调,差异有统计学意义(P<0.01);益气除痰方含药血清组P4HB、Vimentin mRNA的表达量较缺氧模型组明显下调,差异有统计学意义(P<0.01,P<0.05)。结论益气除痰方可抑制缺氧诱导的上皮间质转化,可能与其下调P4HB mRNA表达相关。

胸腺素β_4-脯氨酸寡肽酶-AcSDKP轴在肝内生物学功能的研究

N-乙酰基-丝氨酰-天冬氨酰-赖氨酰-脯氨酸(N-acetyl-Ser-Asp-Lys-Pro AcSDKP)由脯氨酸寡肽酶水解其前体胸腺素β4生成,三者均存在于肝内并发挥重要生物学功能。本文就胸腺素β4-脯氨酸寡肽酶-AcSDKP轴在肝内病理生理功能,特别是其与肝损伤修复和肝脏细胞外基质沉积关系的研究做一概述。

基于生物信息学分析骨肉瘤的关键基因和qRT-PCR实验验证

目的利用生物信息学方法筛选出与骨肉瘤(osteosarcoma,OS)相关的关键基因,以作为OS的潜在诊断标志物和新治疗靶点。方法从基因表达综合(Gene Expression Omnibus,GEO)数据库中检索下载2个符合本研究的OS相关数据集(GSE16088和GSE42572),共包括21例OS组织样本和14例正常骨组织样本。对数据集进行矫正分析鉴定出差异表达基因(differentially expressed genes,DEGs)。通过加权基因共表达网络分析方法(weighted gene co-expression network analysis,WGCNA)与DEGs筛选出交集基因。对交集基因进行疾病本体论(Disease Ontology,DO)、基因本体论(Gene Ontology,GO)、京都基因与基因组百科全书分析(Kyoto Encyclopedia of Genes and Genomes,KEGG)和蛋白互作(protein-protein interaction,PPI)网络分析。采用受试者工作特征(receiver operating characteristic,ROC)曲线评估该PPI网络degree排名前10位的Hubbe基因的表达水平对OS患者的诊断效能,并以另一个OS数据集GSE19276对Hubbe基因进行验证筛选出关键基因。分析关键基因与浸润性免疫细胞的相关性。收集2020年9月1日至2022年6月30日于广西中医药大学第一附属医院住院手术的4例OS患者的OS组织及其癌旁组织,采用实时荧光定量聚合酶链式反应(real-time quantitative polymerase chain reaction,qRT-PCR)对关键基因进行实验验证。结果在OS组织与正常骨组织中共筛选出687个DEGs(上调基因523个和下调基因164个)。WGCNA关键模块基因2338个。DEGs与WGCNA关键模块基因共有交集基因545个。DO富集分析结果表明,DEGs与WGCNA结果的交集基因主要与泌尿系统癌症、肾癌、生殖细胞癌、肌肉骨骼系统癌症和胚胎癌等癌症相关。GO富集结果表明,交集基因主要参与骨化的形成、细胞外基质组织和生物矿物组织发育等生物学过程。KEGG通路富集在磷脂酰肌醇3激酶(phosphatidylinositide 3-kinase,PI3K)/蛋白激酶B(protein kinase B,PKB,又名Akt)信号通路、过氧化物酶体增殖物激活受体(peroxisome proliferators-activated receptor,PPAR)信号通路及流体剪切应力和动脉粥样硬化等信号通路上。PPI网络分析中degree排名前10位的Hubbe基因为磷脂酰肌醇4,5-二磷酸3-激酶催化亚基α(phosphatidylinositol-4,5-bisphosphate 3-kinase catalytic subunit alpha,PIK3CA)、脯氨酰4-羟化酶亚单位α1(prolyl 4-hydroxylase subunit alpha 1,P4HA1)、整合素αⅤ(integrin alphaⅤ,ITGAⅤ)、组蛋白去乙酰化酶2(histone deacetylase 2,HDAC2)、连环蛋白β1(catenin beta 1,CTNNB1)、Ⅲ型胶原蛋白α1(collagen typeⅢalpha 1,COL3A1)、Ⅰ型胶原蛋白α2(collagen typeⅠalpha 2,COL1A2)、转导蛋白β样1X相关蛋白1(transducin beta-like 1X-related protein 1,TBL1XR1)、小核核糖核蛋白多肽G(small nuclear ribonucleoprotein polypeptide G,SNRPG)和Ras相关核蛋白(Ras-related nuclear protein,RAN)。以数据集GSE19276绘制ROC曲线验证Hubbe基因表明,P4HA1和ITGAV的准确度较高(均AUC>0.8且P<0.05)。qRT-PCR实验结果显示,P4HA1和ITGAV mRNA在OS组织中高表达(均P<0.01)。结论P4HA1和ITGAV是OS的潜在生物标志物和治疗靶点。

反义寡脱氧核苷酸对脯氨酰4-羟化酶mRNA表达的抑制作用

目的：观察反义寡脱氧核苷酸（ＯＤＮ）对脯氨酰４－羟化酶（Ｐ４Ｈ）两种亚基ｍ ＲＮＡ 表达的影响。方法：采用定量ＲＴ－ＰＣＲ技术检测培养的人皮肤成纤维细胞中Ｐ４Ｈ ｍ ＲＮＡ的相对含量。结果：不同浓度（０．１，０．２，０．５，１．０ μｍ ｏｌ／Ｌ）反义ＯＤＮ处理组，人皮肤成纤维细胞中Ｐ４Ｈ ｍ ＲＮＡ表达水平均显著低于对照组及错配ＯＤＮ 处理组；其中０．１，０．２ μｍ ｏｌ／Ｌ反义ＯＤＮ作用２０ ｈ 时，抑制效应达到最大，５０～７０ ｈ 后，逐渐恢复到对照组水平。正义ＯＤＮ与错配ＯＤＮ对Ｐ４Ｈ ｍ ＲＮＡ表达则无明显抑制作用。结论：反义ＯＤＮ 对Ｐ４Ｈ 两种亚基的ｍ ＲＮＡ表达均有显著和特异的抑制作用。

表达Ⅰ型类人胶原蛋白和脯氨酰4-羟化酶α-蛋白的转基因家蚕品系构建

家蚕丝腺具有高效合成与分泌蚕丝蛋白质的能力,探究利用转基因方法开发家蚕丝腺为生物反应器生产高附加值外源蛋白质的技术途径。将Ⅰ型类人胶原蛋白基因(HCool-Ⅰ)和胶原蛋白羟基化修饰所必需的脯氨酰4-羟化酶α-亚基基因(BmP 4Hα)通过piggyB ac转座子及显微注射方法,同时转入家蚕早期胚胎,在丝素轻链基因fib-L启动子驱动下转入的2个外源基因在家蚕幼虫后部丝腺获得表达。利用反向PCR和生物信息学等方法鉴定、分析转基因家蚕基因组中有19个外源piggyB ac的整合位点,分别位于基因的外显子区域、内含子区域和基因间区,可定位至家蚕的15条染色体上。实时荧光定量PCR检测不同整合位点的转基因家蚕品系幼虫后部丝腺中HCool-Ⅰ基因mRNA转录量存在极显著差异,转录量最高和最低的品系间相差23倍左右;转基因家蚕后部丝腺中BmP 4Hα基因mRNA的转录量比野生型家蚕高出2万多倍。利用SDS-PAGE检测转基因家蚕G3代5龄5 d幼虫的后部丝腺总蛋白质在55 kD和64 kD处分别存在特异性蛋白条带,表明BmP 4Hα和HCool-Ⅰ蛋白已在G3代转基因家蚕丝腺中获得表达。

Expression of Prolyl 4-Hydroxylase Beta-Polypeptide in Non-Small Cell Lung Cancer Treated with Chinese Medicines

Objectives： To investigate the role of prolyl 4-hydroxylase beta polypeptide （P4HB） expressed in lung carcinoma and the intervention effect of Yiqi Chutan Formula （益气除痰方, YQCTF）. Methods： Lung carcinoma model was established by subcutaneously inoculating LEWIS lung carcinoma cells in C57BL/6J mice. The differential expression of P4HB protein between the YQCTF （3.0 g/kg, gavage, once daily, 21 days） group and the control group was acquired by a 2 fluorescence difference gel electrophoresis （2D-DIGE）, verified by Westem blotting and identified by matrix-assisted laser desorption ionization time of flight mass spectrometry （MALDI-TOF/＇IOF-MS）. The expression of P4HB and P4HB mRNA in cultured A549 cells from cisplatin （DDP） 1.5μg/mL group and 15% serum combined with DDP 1.5 μg/mL group were detected by cellular immunohistochemistry and reverse chain reaction, respectively. Results： The proteomics research discovered that one-third of differential proteins including P4HB were decreased in the YQCTF group （P〈0.01）. Clinical pathology and tissue microarray studies showed that P4HB expression in lung cancer tissue was stronger than adjacent tissues and normal lung epithelial （P〈0.01）. In the YQCTF and DDP combined groups, the expression of P4HB and P4HB mRNA in A549 cell were decreased significantly （P〈0.01）. Conclusion： YQCTF could inhibit the LEWIS lung carcinoma＇s growth, decrease the expression of P4HB in LEWIS lung carcinoma and A549 cells. YQCTF might take effect through regulating P4HB in endoplasmic reticulum to inhibit the incidence and growth process of lung cercinoma.

P4HA2通过激活PI3K/AKT/mTOR信号通路促进肝癌的发生和发展

目的 探讨脯氨酸4-羟化酶Ⅱ(P4HA2)在肝癌细胞发生发展中的作用及相关机制。方法 利用GEPIA、Human Protein Atlas数据库预测P4HA2在肝癌中的表达情况,利用K-M plotter在线数据库分析P4HA2的表达情况与肝癌预后的关系,采用qRT-PCR和Western blot检测肝癌细胞和正常肝细胞中P4HA2的表达。构建慢病毒载体,用携带P4HA2 shRNA和Con shRNA的慢病毒载体分别转染肝癌SNU-449和Hep-3B细胞系,建立沉默表达P4HA2的细胞株(shP4HA2组)和对照组细胞株(NC组)。采用CCK-8、集落形成试验、划痕实验和Transwell实验分别检测细胞增殖、迁移和侵袭能力。采用Western blot实验检测上皮-间质转化和PI3K/Akt/mTOR信号通路相关蛋白表达情况。结果 在线数据库分析结果显示,肝癌组织中P4HA2表达高于正常肝组织(P<0.05)。同时,肝癌细胞系中P4HA2 mRNA和蛋白表达水平也高于正常肝细胞(P<0.01)。慢病毒干扰后,与NC组相比,shP4HA2组中mRNA和蛋白表达水平下降(P<0.05)。P4HA2基因表达沉默后,细胞的增殖、迁移和侵袭受到抑制。Western blot显示,相对于NC组,shP4HA2组的E-cadherin蛋白表达上升,N-cadherin、Snail蛋白表达下降(P<0.05),在PI3K/AKT/mTOR通路中,磷酸化的PI3K(P-PI3K)、AKT(P-AKT)和m TOR(P-mTOR)显示出较低的水平(P<0.05)。结论 P4HA2通过激活PI3K/Akt/mTOR信号通路影响肝癌细胞的增殖、迁移、侵袭,促进肝癌的发生发展。

脯氨酰-4-羟化酶基因在妊高征胎盘中的表达及其临床意义

目的 :通过检测脯氨酰 4 羟化酶 (P4H)基因在妊娠高血压综合征 (妊高征 )患者胎盘中的表达 ,了解其在妊高征病理生理机制中的作用 .方法 :采用半定量RT PCR技术检测1 0例正常妊娠妇女 (对照组 )及 1 0例中、重度妊高征患者 (妊高征组 )胎盘组织P4H和 β actinmRNA水平 .结果 :P4H与 β actin积分吸光度比值在对照组和妊高征组胎盘组织中分别为 :0 .386 82± 0 .0 7931 ;0 .4 5 6 71± 0 .0 5 80 3.显示P4HmRNA在对照组和妊高征组胎盘组织中均有表达 ,妊高征组胎盘组织P4H基因的表达明显高于对照组 ,差异有显著性 (P =0 .0 37) .结论 :妊高征患者胎盘组织中P4H基因的高表达 ,可能是妊高征一系列病理生理变化的环节之一 .

ING4、PHDs以及HIF-1α在低氧性肺动脉高压大鼠中的表达变化

目的研究大鼠低氧性肺动脉高压(hypoxic pulmonary hypertension,HPH)模型中ING4表达变化的规律及其与PHDs、HIF-1α间的相互关系。方法实验复制HPH大鼠模型,在缺氧不同时间点,测定大鼠平均肺动脉压(mPAP)及右心室肥大指数(RVHI),HE染色观察肺小动脉重塑(HPVR)。原位杂交、RT-PCR、检测肺内ING4、PHD1、PHD2、PHD3及HIF-1α的mRNA表达水平及部位,免疫组化、Western blot检测以上蛋白质表达水平及部位。结果 (1)缺氧7d后大鼠的mPAP开始上升,与对照组比较有显著性差异(P<0.05),缺氧14d后出现肺血管重塑和RVHI增加,与对照组比较有显著性差异(P<0.05)。HIF-1α蛋白在缺氧3d组表达均开始升高(P<0.05,与对照组比),缺氧7d达高峰,14d和21d稍下降。HIF-1αmRNA在缺氧14d后表达略增高(与对照组比较P<0.05)。(2)对照组PHD1蛋白质呈阳性表达,缺氧14d下降,缺氧21d保持较低水平。PHD1mRNA表达差异无显著性。对照组PHD2蛋白质和mRNA呈阳性表达,缺氧3d增高,缺氧14d达高峰,缺氧21d保持较高水平。对照组PHD3蛋白质呈弱阳性表达,缺氧3d明显增高,缺氧7d保持高水平,缺氧14d和21d下降。对照组肺小血管PHD3mRNA缺氧3d后迅速增高,缺氧14d达高峰,缺氧21d保持高水平。(3)对照组ING4蛋白质呈弱阳性表达,缺氧3d和7d后表达增高,缺氧14d达高峰,缺氧21d稍有下降。对照组ING4mRNA呈阳性表达,缺氧7d组比表达显著增高,直线相关分析表明,在缺氧组大鼠中ING4蛋白质与HIF-1α蛋白质及mPAP、RVHI、WA%负相关。结论肺动脉高压大鼠模型中ING4、PHDs和HIF-1α的表达变化,可能在HPH的发生和发展中发挥作用。

脯氨酸羟化酶GhP4H2在棉花纤维发育中的功能研究

阿拉伯半乳聚糖蛋白(arabinogalactan proteins,AGP)在棉花纤维发育过程中发挥重要作用。AGP由富含羟脯氨酸的主链蛋白和大量Ⅱ型阿拉伯半乳聚糖(arabinogalactan,AG)侧链组成,其合成过程要经历2次翻译后修饰,首先是氨基酸主链上的脯氨酸被脯氨酸羟化酶(prolyl-4-hydroxylases,P4H)羟基化,随后在糖基转移酶(glycosyltransferases,GT)催化作用下将阿拉伯半乳聚糖或寡糖添加到羟脯氨酸残基上。我们前期利用P4Hs的抑制剂处理棉花离体胚发现,棉纤维伸长受到抑制,暗示P4H参与棉纤维生长发育过程。为深入研究P4H在棉纤维发育中的功能,我们从棉花中分离鉴定了1个在棉纤维发育过程中高量表达的脯氨酸羟化酶基因GhP4H2。本研究分别构建了GhP4H2过表达和RNA interference(RNAi)载体,通过农杆菌介导法转化棉花,获得转基因植株,发现过表达转基因棉花株系T_(1)~T_(3)代成熟棉纤维变短,AGP含量增加,AG多糖侧链也发生变化。对过表达转基因植株和野生型植株棉纤维的转录组分析表明,GhP4H2正调控包括AGP在内的细胞壁糖蛋白基因的表达。基于以上研究,我们推测GhP4H2可能主要通过影响AGP糖链组分调控棉纤维生长发育。

千层纸素A通过调控P4HB蛋白介导的hedgehog信号抑制肝癌血管生成

目的:探讨脯氨酸4-羟化酶β亚基(P4HB)蛋白在千层纸素A抗肝癌血管生成中的作用及其可能的机制。方法:Western blot检测6株人肝癌细胞系HCCLM3、Huh7、HepG2、MHCC97-L、Bel-7402及SMMC-7721中P4HB的蛋白表达。MTS试剂盒检测受试化合物对SMMC-7721细胞体外增殖的影响;LDH检测受试化合物对SMMC-7721细胞毒性影响;Western blot法检测受试化合物对SMMC-7721细胞中P4HB蛋白表达的影响;构建P4HB干扰质粒并转染SMMC-7721细胞,Western blot检测干扰转染效率;采用小管形成实验研究干扰P4HB对SMMC-7721细胞血管生成的影响;采用Western blot检测干扰P4HB对SMMC-7721细胞中hedgehog (Hh)信号相关蛋白Patched、Smo及Hhip蛋白表达影响;采用ELISA试剂盒检测激动Hh信号对P4HB蛋白调控SMMC-7721细胞血管内皮生长因子(VEGF)及血小板衍生生长因子(PDGF)分泌影响。结果:6株细胞中,SMMC-7721细胞表达P4HB蛋白最高。与对照组相比,千层纸素A体外可显著抑制抑制SMMC-7721细胞的增殖(P<0.05),并在100μmol·L^(-1)以上时对细胞显示毒性作用(P<0.05)。与对照组相比,千层纸素A可显著抑制SMMC-7721细胞中P4HB蛋白表达(P<0.05);与对照干扰组相比,P4HB干扰质粒可显著抑制SMMC-7721细胞中P4HB蛋白表达(P<0.05),表明质粒构建成功;与对照干扰组相比,干扰P4HB可抑制SMMC-7721细胞的血管生成(P<0.05),降低SMMC-7721细胞Patched及Smo的蛋白表达(P<0.05),并升高Hhip蛋白表达(P<0.05)。此外,与对照组相比,千层纸素A亦能够抑制SMMC-7721细胞Patched及Smo的蛋白表达(P<0.05),并增加Hhip蛋白表达(P<0.05)。与P4HB干扰组相比,激动Hh信号可减弱P4HB干扰所致的细胞VEGF及PDGF分泌下降的作用(P<0.05)。结论:千层纸素A能够通过抑制P4HB介导的hedgehog信号抑制肝癌细胞的血管生成。千层纸素A是抗肝癌血管生成疗法的潜在化合物。

QUANTIFICATION OF P4HA2 mRNA OF FIBROBLASTS WITH SYBR GREEN BASED RT-PCR FOR CORRECTING CMV INACTIVATION EFFICIENCY IN DONOR BLOOD

Objective To quantify proline 4-hydroxylase, alpha polypeptide ii （ P4HA2 ） mRNA of human embryo lung fibroblast （HELF） with SYBR green based reversed transcript PCR （RT-PCR） for correcting cytomegalovirus （CMV） inactivation or clearance efficiency in donor blood. Methods A pair of specific primers of exon 12a of P4HA2 was designed, and the related PCR-reaction system and condition were optimized. Then the recombinant plasmid containing the target fragment was constructed for making standard curve with SYBR green based real-time RT-PCR. Finally, the sensitivity, reproducibility, and specificity of this method were fully estimated. Results The sensitivity of the method was 1.5E ＋ 04 copies/mL of P4HA2 mRNA, corresponding to 10^3 fibroblasts. In addition, existence of 8. 67E ＋ 06 leukocytes could not interfere with the accurate quantification of HELF in the large dynamic range. The intra-assay variability and inter-assay variability both varied in different concentrations, being higher in low concentrations and lower in high concentrations. But all of them were below 13. 76% in variation, which showed acceptable stability of this method. Conclusion SYBR green and specific primer based real-time RT-PCR show up a good quality for quantifying HELF P4HA2 mRNA with good specificity, stability, and high sensitivity. Approximate 10 copies of P4HA2 mRNA per cell in average can be detected by the method. Therefore, this method can be used to deduct fibroblast-associated CMV for correcting CMV inactivation efficiency in leukocytes.

氨酰4-羟化酶A2通过抑制炎症反应缓解肾纤维化

目的:利用体内和体外模型探讨氨酰4-羟化酶A2(P4HA2)对肾间质纤维化的作用及其机制。方法:采用输尿管结扎模型构建动物肾纤维化,使用免疫组化技术检测P4HA2表达水平;采用不同梯度浓度TGF-β刺激HK2细胞构建细胞肾纤维化模型,利用免疫印迹和细胞免疫荧光检测P4HA2蛋白表达变化水平;利用腺病毒转染HK2细胞,使用免疫印迹和酶联免疫吸附试验技术探索P4HA2在细胞水平对NF-κB信号通路和下游炎症因子的影响。结果:与假手术组小鼠比较,模型组小鼠P4HA2表达量显著增加,且集中于肾小管细胞胞质与胞核中。使用50 ng/mL TGF-β刺激HK-2细胞24 h后P4HA2表达水平显著升高,且细胞形态由鹅卵石形变成针尖样长梭形;与转染对照组(scramble)比较,sh-P4HA2抑制NF-κB信号通路相关蛋白表达量,减少下游炎症因子IL-1β、IL-6和TNF-α水平。结论:P4HA2可能调控NF-κB信号通路,抑制机体炎症反应,缓解肾间质纤维化发展。

正常孕妇和子前期患者胎盘缺氧诱导因子脯氨酸羟化酶的表达

目的分析正常孕妇和子前期患者胎盘组织缺氧诱导因子脯氨酸羟化酶(HPH)mRNA的表达,探讨子前期胎盘缺氧的发生与滋养叶细胞氧敏感性的关系。方法行剖宫产分娩或接受计划生育手术的孕妇共66名,分为早孕组(n=13)、中孕组(n=9)、晚孕组(n=13,作为子前期组和妊娠期高血压组的对照)、子前期组(n=20)和妊娠期高血压组(n=11)。采用原位杂交和Real-Time PCR技术对胎盘或绒毛组织中HPH-1、-2、-3 mRNA的表达进行定位和定量检测。结果 HPH-1、-2、-3 mRNA主要在胎盘滋养叶细胞的细胞质内表达,HPH-1 mRNA在绒毛外滋养叶细胞的细胞质内呈强特异性表达。随着妊娠进展,HPH-1 mRNA表达量明显增加(r=0.616,P<0.001)。子前期组HPH-1 mRNA表达量显著低于晚孕组(P<0.05);妊娠期高血压组HPH-1 mRNA表达量也低于晚孕组,但差异无统计学意义(P>0.05)。子前期组患者胎盘质量与HPH-1 mRNA表达量呈正相关(r=0.457,P<0.05)。结论子前期患者滋养叶细胞氧敏感性降低(HPH-1 mRNA低表达)是导致胎盘缺氧表现(缺氧反应途径过度激活)的重要原因。