Carboxyl Terminus Truncated Human Papillomavirus Type 58 L1 Protein Maintains Its Bioactivity and Ability to Form Virus-like Particles

Summary: To prepare carboxyl terminus truncated human papillomavirus type 58 L1(HPV58L1) protein and evaluate its ability to form virus-like particles, the baculovirus and Sf-9 insect cells was used to express HPV58L1 protein, and pFastBac-Htb containing HPV58L1 gene sequence of carboxyl terminus truncation was generated. Then Sf-9 cells were infected with recombinant baculovirus. After being cultured, the post-infected cells expressing-HPV58L1 protein-were harvested and analyzed by SDS-PAGE and Western blot. The ProBond~TM purification system was used for protein purification. The bio-activity of purified protein was identified by mouse erythrocyte hemagglutination assay, and the VLP formation was examined with transmission electron microscope. Our results showed that the recombinant baculovirus was generated and the Sf-9 cells was infected with the recombinant baculovirus, and after collecting, total cellular proteins were extracted. Truncated HPV58L1 protein with MW 58KD was revealed by SDS-PAGE and confirmed by Western blot. The purified L1 proteins under native condition could cause mouse erythrocytes to agglutinate and form VLP. It is concluded that HPV58L1 protein with carboxyl terminus truncation could be efficiently expressed. In baculovirus Sf-9 cells expression system, the purified protein could self-assemble into virions in vitro, and induce agglutination of mouse erythrocytes, indicating that carboxyl terminus truncation does not interfere with the bioactivity of HPV58L1 protein.

MAPPING EPITOPES OF HUMAN PAPILLOMAVIRUS TYPE 16 L1 PROTEIN WITH A PHAGE DISPLAY EPITOPE LIBRARY

The objective of this study is to map epitopes on HPMAPV16 L1 protein and provide information to the design of HPV16 prophylactic peptide vaccine. The epitopes on L1 protein were screenedby polyclonal and two monoclonal antibodies (BS and F4G3) against RPV16 L1 protin from a 6-merfd phage display epitope library with the method or immuuo-afrinity screening (Biopauuing). Aferthree rounds or Bio-Panning, the Positive phages were detected by L1 antibodies again with ELISA.The positive phages reacted strongly with L1 antibodies were then identified by DNA sequencing.Three mimotopes have been screened by polycloual and two monoclonal antibodies. The mimotope(LSLFSC) reacted with mouoclonal antibody B8 showed 50% pomology with the sequence 270275a. a (DSLFFY) of prototype HPV16 L1. Another mimotope (LTSSYS) reacted with polyclonalantibodies had 66% pomology with the L1 sequence 516~521a. A(TTSSTS), also a mimotope (DRWDRF) was found had the bomologic RF with the known L1 sequence 441 ~446a. a. The mimotopesLSLFSC and DRWDRF were adjacent to the epitopes at 267~269a. a and 422~441 a. a reported byother researchers Previously. Our results suggest that there might be a batch of epitopes on HPV16L1 ppotein, and the predominant epitopes of HPV16 L1 protein are located in the above two domains. These results will be helpful for design or HPV16 prophylactic peatide vaccines and HPVpolyvalent vaccines.

PD-1、PD-L1、MMR蛋白在子宫内膜癌中的表达及与患者临床病理特征的相关性

目的:探讨程序性死亡受体1(PD-1)、程序性死亡配体1(PD-L1)、错配修复(MMR)蛋白(MLH1、PMS2、MSH2和MSH6)在子宫内膜癌中的表达及与患者临床病理特征的相关性。方法:选取我院2020年6月—2023年6月收治的80例子宫内膜癌患者作为研究对象,取患者的子宫内膜组织进行免疫组化检测,检测PD-1/PD-L1、MMR蛋白表达水平。并分析不同病理特征子宫内膜癌患者PD-1、PD-L1表达情况与MMR蛋白缺失情况,最后采用Spearman相关法分析PD-1、PD-L1、MMR蛋白与子宫内膜癌临床病理特征的相关性。结果:80例子宫内膜癌患者中,子宫内膜癌组织PD-1阳性表达率为63.75%,PD-L1阳性表达率为67.50%;MMR蛋白表达缺失率为70.00%;80例子宫内膜癌患者中,PD-1、PD-L1阳性与阴性患者的细胞分化程度、FIGO分期、子宫肌层浸润、淋巴结转移情况对比差异显著,此外PD-L1阳性与阴性病理类型对比差异显著(P<0.05),MMR蛋白基因缺失与基因完整患者的肿瘤部位、细胞分化程度、子宫肌层浸润、淋巴结转移情况对比差异显著(P<0.05);PD-1与子宫内膜癌细胞分化程度、FIGO分期、子宫肌层浸润、淋巴结转移呈正相关,PD-L1与病理类型、细胞分化程度、FIGO分期、子宫肌层浸润、淋巴结转移呈正相关,MMR蛋白与子宫内膜癌肿瘤部位、细胞分化程度、子宫肌层浸润、淋巴结转移呈正相关(P<0.05)。结论:PD-1、PD-L1、MMR蛋白表达与子宫内膜癌患者的临床病理特征具有密切关系,临床可考虑应用三者对子宫内膜癌的诊断与预后进行评价,为临床提供参考意义。

基于PD-L1蛋白表达水平的胃癌免疫治疗专家共识(2023年版)

以程序性死亡蛋白-1(programmed death protein-1,PD-1)抑制剂为代表的免疫检查点抑制剂在胃癌中显示良好疗效,逐步改变晚期胃癌的治疗格局。对于程序性死亡蛋白配体-1(programmed death-ligand 1,PD-L1)高表达的患者,PD-L1单抗的治疗效果更为优异,且与PD-L1蛋白表达水平呈正相关。而对于PD-L1阴性或低表达这类免疫治疗非优势人群,以PD-1单抗为基础的用药方案疗效有限,尝试双特异性抗体、ADC等不同药物的联合也是一种趋势。为了精准指导临床实践,中国抗癌协会胃癌专业委员会组织国内胃癌领域专家进行多轮讨论,系统汇总国内外最新指南和循证证据,并结合我国临床实际,从病理检测、晚期治疗以及围术期治疗3个方面制订了本专家共识,旨在提高胃癌诊治的科学性和规范性,尤其是指导基层医生对免疫治疗的选择和应用。

UCH-L1、PRDX1与AIS患者阿替普酶治疗效果的关系

目的研究泛素羧基末端水解酶L1(ubiquitin carboxyl terminal hydrolase L1,UCH-L1)、过氧化还原蛋白1(peroxiredox protein 1,PRDX1)与急性缺血性脑卒中(acute ischemic stroke,AIS)患者阿替普酶治疗效果的关系。方法选取2020年6月至2022年6月嘉兴市第一医院收治的198例AIS患者作为研究组,选取同期100名健康体检者作为健康组,利用酶联免疫吸附试验(enzyme linked immunosorbent assay,ELISA)检测血清UCH-L1、PRDX1水平。AIS患者均使用阿替普酶静脉溶栓治疗,治疗10d后评价临床疗效,比较不同疗效患者临床资料及血清UCH-L1、PRDX1水平差异,分析UCH-L1、PRDX1与阿替普酶治疗效果的关系。结果研究组患者的UCH-L1、PRDX1水平高于健康组(P<0.05)。重症AIS患者的UCH-L1、PRDX1水平高于中症、轻症患者(P<0.05)。完全前循环梗死型AIS患者的UCH-L1、PRDX1水平高于腔隙性梗死、后循环梗死、部分前循环梗死型(P<0.05)。AIS患者阿替普酶治疗后UCH-L1、PRDX1水平低于治疗前,且阿替普酶治疗效果越差UCH-L1、PRDX1水平越高(P<0.05)。UCH-L1、PRDX1联合预测AIS患者阿替普酶治疗效果的效能优于单一预测(P<0.05)。年龄、疾病严重程度、入院时美国国立卫生研究院卒中量表评分、UCH-L1、PRDX1是影响AIS患者阿替普酶治疗效果的危险因素(P<0.05)。结论UCH-L1、PRDX1水平在AIS患者血清中升高,与患者疾病严重程度、脑卒中分型有关,是影响AIS患者阿替普酶治疗效果的危险因素,可用于阿替普酶治疗效果的早期预测。

胶质纤维酸性蛋白、泛素羧基端水解酶L1联合卒中量表评分在急性脑梗死预后评估中的应用研究

目的探讨胶质纤维酸性蛋白(GFAP)、泛素羧基端水解酶L1(UCH-L1)联合美国国立卫生研究院卒中量表(NIHSS)对急性脑梗死(ACI)预后的预测价值。方法收集我院124例ACI患者资料(ACI组)及66例正常人(健康组)。比较两组GFAP、UCH-L水平变化;分析不同预后ACI患者GFAP、UCH-L水平及与NIHSS评分的关系;探讨上述指标在ACI治疗预后评估中的价值。结果ACI组GFAP、UCH-L水平及NIHSS评分显著高于健康组,预后良好组GFAP、UCH-L水平及NIHSS评分显著低于预后不良组(P<0.05)。GFAP、UCH-L水平与NIHSS评分、mRS评分均呈正相关关系(P<0.05)。ROC结果示,GFAP、UCH-L及NIHSS评分联合检测AUC为0.774,明显高于各项指标单独检测(P<0.05)。结论GFAP、UCH-LI、NIHSS评分可作为评估ACI患者预后的参考指标,且上述指标联合预测价值更高。

Novel heat shock protein Hsp70L1 activates dendritic cells and acts as a Th1 polarizing adjuvant

Heat shock proteins (HSPs) are reported to act as effective adjuvants to elicit anti-tumor and anti-infection immunity. Here, we report that Hsp70-like protein 1 (Hsp70L1), a novel HSP derived from human dendritic cells (DCs), has potent adjuvant effects that polarize responses toward Th1. With a calculated molecular weight of 54.8 kDa, Hsp70L1 is smaller in size than Hsp70 but resembles it both structurally and functionally. Hsp70L1 shares common receptors on DCs with Hsp70 and can interact with DCs, promoting DC maturation and stimulating secretion of the proinflammatory cytokines interleukin 12p70 (IL-12p70), IL-1beta, tumor necrosis factor-alpha (TNF-alpha), and the chemokines IP-10, macrophage inflammatory protein-1alpha (MIP-1alpha), MIP-1beta, and normal T cell expressed and secreted (RANTES). The induction of interferon-gamma-inducible protein 10 (IP-10) secretion by Hsp70L1 is not shared by Hsp70, and other functional differences include more potent stimulation of DC IL-12p70, CC-chemokine, and CCR7 and CXCR4 expression by Hsp70L1. Immunization of mice with the hybrid peptide Hsp70L1-ovalbumin(OVA)(257-264) induces an OVA(257-264)-specific Th1 response and cytotoxic T lymphocyte (CTL) that results in significant inhibition of E.G7-OVA tumor growth. The ability of Hsp70L1 to activate DCs indicates its potential as a novel adjuvant for use with peptide immunizations; the Hsp70L1 antigen peptide hybrid may serve as a more effective vaccine for the control of cancer and infectious diseases.

Research Progress of HPV L1 Capsid Protein in Prediction of Cervical Lesions

Cervical cancer is one of the most common malignant gynecological tumors and has the second highest incidence of all malignancies in females.Chronic and persistent infection with High Risk Human Papillomavirus(HR-HPV)is the main cause of cervical cancer.There is a distinct lack of methodology by which to determine whether cervical epithelial dysplasia is cancerous following HPV infection.HPV L1 capsid protein is a major structural protein of human papillomavirus(HPV),and it is the main target of the local cellular immune response aiming to combat human papillomavirus after HPV infection within cervical cells.Greater understanding of HPV L1 capsid protein and its association with cervical cytology,histopathology,patient age and human papillomavirus viral load has the potential to contribute toward improved the diagnosis and management of cervical cancer,providing useful information for gynecological clinicians in the hope of improving patient treatment and quality of life.This article reviews the predictive utility of HPV L1 capsid protein for cervical lesions.

Positive Correlation between PMS2 Deficiency and PD-L1 Expression in Pancreatic Cancer

Background: Pancreatic cancer is one of the most lethal types of cancer, and immunotherapy has become a promising remedy with advancements in tumor immunology. However, predicting the clinical response to immunotherapy in pancreatic cancer remains a dilemma for clinicians. Methods: GEPIA database was used to analyze the differential expression of MMR and PD-L1 genes in 33 common cancer types including pancreatic cancer. The expression levels of MMR and PD-L1 genes were downloaded from the GEPIA and GEO databases to analyze the correlation between MMR genes and PD-L1, and the clinicopathological and survival information were downloaded from the TCGA databases to analyze the relationship between the expression of MMR, PD-L1 and clinicopathological characteristics, prognosis. Meanwhile, the tumor tissue samples of 41 patients with pancreatic cancer were collected, and the protein expression levels of MMR and PD-L1 were detected by immunohistochemical assay. Furthermore, we analyzed the correlation between MMR and PD-L1, and the correlation between the expression of MMR, PD-L1 and clinicopathological characteristics, prognosis of pancreatic cancer patients. Results: Bioinformatics analysis showed that MLH1, MLH3, MSH2, MSH3, and PMS2 were highly expressed in most cancer types including pancreatic cancer (P P = 0.012), clinical stage (I vs II: P = 0.016), MSH2 expression was related to clinical stage (P < 0.05), T stage (T3 vs T4: P = 0.039), and MSH3 expression was related to T stage (P < 0.05). Besides, both MSH2 expression (P P = 0.044) were significantly associated with prognosis. GEPIA data also showed that MSH2 expression was related to prognosis (P = 0.008). The correlation analysis revealed that the expressions MSH2, MLH1, PMS2 had strong correlations with PD-L1 both in GEPIA and GEO databases. Real-world data indicated that of the 41 pancreatic cancer patients, 5 cases had MLH1 deletion, 5 cases had MSH2 deletion, 4 cases had PMS2 deletion, and 12 cases had PD-L1 positive expression. Notably, PMS2 deletion was associated with PD-L1 positive expression (P = 0.035). In addition, MLH1 was related to clinical stage (P = 0.033), age (P = 0.048), and MSH2 was related to clinical stage (P = 0.033). However, MLH1 (P = 0.697), MSH2 (P = 0.956), PMS2 (P = 0.341), and PD-L1 (P = 0.734) appeared to have no impact on overall survival among patients with pancreatic cancer. Conclusion: Both bioinformatics and real-world data showed that there were correlation between PMS2 deletion and PD-L1 expression, and correlation between MLH1, MSH2 and clinical stage.

素馨花水提物及其主要成分对3T3-L1细胞成脂分化的影响

该研究探讨素馨花水提物(WE)及其化学成分在3T3-L1前脂肪细胞上的降脂作用。通过将3T3-L1细胞诱导为成熟脂肪细胞,油红O染色定量和检测甘油三酯(TG)含量判断素馨花样品对脂滴的抑制作用;液质联用仪分析WE中化学成分;MTT检测素馨花及其成分对3T3-L1细胞增殖的影响;Western Blot检测AMPK、C/EBPα、FAS、ACC、CPT1、Bax、Bcl-2等蛋白表达。结果发现,WE能剂量依赖性抑制脂滴形成,其中高浓度WE(500μg/mL)能降低中性脂质含量23.59%,降低TG含量30.20%,在脂肪积累早期作用最显著,并证明其活性成分主要是橄榄苦苷,含量为13.77%。WE及橄榄苦苷能激活AMPK(123.19%和115.98%)和其下游靶点ACC(451.06%和1050.0%)的磷酸化、下调其下游靶点FAS(81.72%和60.50%)的蛋白表达,减少脂肪形成,提高CPT1(164.84%和292.19%)蛋白的表达,加快脂肪酸氧化;抑制C/EBPα(68.97%和34.57%)的表达,影响3T3-L1细胞分化;上调Bax(154.60%和139.37%)、下调Bcl-2(41.10%和45.62%)蛋白的表达,诱导脂肪细胞凋亡。结果提示,WE能在3T3-L1细胞分化过程早期抑制细胞生长、分化和脂肪合成并促进脂肪酸氧化从而有效抑制脂质积累,机制上可能通过调控AMPK和Bax/Bcl-2通路。

子宫颈病变中HPV L1蛋白和p16的表达

目的研究HPV L1蛋白和p16在子宫颈各种病变中的表达情况,探讨它们在子宫颈病变进展中的预测价值。方法应用免疫组化方法检测41例各种子宫颈病变(CIN1级18例、CIN2级9例、CIN3级8例和浸润性鳞状细胞癌6例)中HPV L1蛋白和p16的表达。结果HPV L1蛋白在各种子宫颈病变中的阳性率为26.8%。其中HPV L1在CIN1中的阳性表达率为38.9%,CIN2为44.4%,CIN3和浸润性鳞状细胞癌均无表达。p16在各种子宫颈病变中的阳性率为68.3%,其在CIN1中的阳性表达率为38.9%,CIN2为77.8%,CIN3和浸润性鳞状细胞癌均表达阳性。100%CIN3和浸润性鳞状细胞癌为p16+/HPV L1-,而61.1%CIN1中为p16-/HPV L1+或p16-/HPV L1-。结论随着子宫颈病变的进展,HPV L1阳性表达率降低而p16阳性表达率增高。p16+/HPV L1-提示子宫颈鳞状上皮内瘤变有进展的可能,而p16-/HPV L1+和p16-/HPV L1-可能为无进展的或潜在消退的子宫颈病变。

人乳头瘤病毒16型L1蛋白B细胞表位预测

目的预测人乳头瘤病毒16型L1（HPV-16 L1）蛋白的B细胞表位。方法先从NCBI的蛋白质数据库中获得HPV-16 L1蛋白的氨基酸序列,再采用DNAStar中的Protean模块分析HPV-16型L1蛋白的二级结构、柔韧性、亲水性、表面可及性以及抗原性,然后结合吴玉章等建立的氨基酸抗原性指数方法计算其平均抗原指数（AI）,综合分析上述多个参数,预测其可能的B细胞表位区域,并用在线BLAST进行同源性匹配分析。结果综合分析多个参数,预测得出HPV-16 L1蛋白的B细胞表位可能位于第51～58、87～97、214～220、290～296、335～341、351～366、408～418、430～442和475～496肽段,进一步的同源性匹配分析显示肽段51～58、335～341、351～366、408～418、430～442以及475～496为其B细胞表位优势区域,其中肽段51（PIKKPNNN）58、351（SETTYKNTNFKEYLRH）366、408（PPPGGTLEDTY）418和430（KHTPPAPKEDPLK）442的氨基酸序列为HPV-16型L1蛋白所特有,而肽段475（KAKPKFTLGKRKATPTTSSTST）496与HPV-16 E1蛋白具有同源性、335（DTTRSTN）341的氨基酸序列与很多其他型别的HPV的L1蛋白具有同源性。结论综合多种方案预测得到HPV-16 L1的多个B细胞表位优势区域。

PD-L1分子在肺癌细胞株上的表达及其生物学意义

背景与目的目前研究表明,多种人类肿瘤大量表达的PD-L1分子参与了肿瘤免疫逃逸,其机制主要在于肿瘤细胞通过高表达PD-L1分子,与T细胞上的受体PD-1的结合,传递负性调控信号,导致肿瘤抗原特异性T细胞的凋亡和免疫无能。本文着重探讨PD-L1分子在肺癌细胞株上的表达及其对T细胞杀伤效应的调节作用。方法采用常规方法从健康人外周血单个核细胞诱导DCs,并经凋亡肿瘤细胞和激发型CD40单克隆抗体刺激获得成熟DCs,与自体T细胞共育后获得肿瘤特异性CTL细胞;流式细胞术检测肺癌细胞上PD-L1分子的表达;JAM法和单抗阻断实验分析CTL细胞对肺癌细胞株的杀伤效应,ELISA法检测细胞培养上清中IFN-γ的含量。结果经凋亡肿瘤细胞负载的成熟DCs可诱导自体T细胞分化为肿瘤特异性CTL;H1299高表达PD-L1分子(90.3±4.2)%,而A549低表达PD-L1分子(19.4±5.2)%;CTL对A549具有高效特异的杀伤力,而对H1299不能高效杀伤;联合应用PD-L1单抗可促进CTL对H1299的杀伤作用和IFN-γ的分泌(P<0.05)。结论在肺癌细胞株上表达的PD-L1分子,可降低CTL对肺癌细胞的杀伤效应。

HPV L1壳蛋白与p16^(INK4a)的免疫组化检查在宫颈病变诊断中的应用

目的检测宫颈上皮病变过程中HPV L1壳蛋白和p16INK4a蛋白的表达,探讨二者联合在宫颈病变诊断中的应用价值。方法用免疫细胞化学方法检测169例不同级别的宫颈液基细胞学标本中HPVL1壳蛋白和p16INK4a蛋白的表达,并与组织病理学检查结果比较。结果随着宫颈活检病理分级升高,HPV L1壳蛋白阳性[L1(+)]率降低(P<0.01),p16INK4a阳性[p16(+)]率升高(P<0.01)。HPVL1壳蛋白阳性率与病理分级呈负相关(rs=-0.436,P<0.01);而p16INK4a阳性率与病理分级呈正相关(rs=0.459,P<0.01)。在宫颈上皮内瘤变(CIN)CIN1、CIN2、CIN3及鳞状细胞癌(SCC)中,L1(+)/p16(-)的表达率分别为19.18%、2.44%、0.00%、0.00%,L1(-)/p16(+)表达率分别为30.14%、75.61%、92.86%、100.00%。L1、p16INK4a、L1(-)/p16(+)在CIN1的表达与CIN2、CIN3、SCC比较,差异均具有统计学意义(P<0.01)。结论HPV L1壳蛋白、p16INK4a均可作为诊断宫颈病变程度的生物学标志;而HPV L1壳蛋白联合p16INK4a不仅能够预测宫颈病变的程度,而且有利于对CIN1患者的随访,可为宫颈癌早期诊断提供新的指标。

血清4型禽腺病毒胶体金免疫层析检测方法的建立

为建立对血清4型禽腺病毒(FAdV-4)进行快速检测的胶体金免疫层析法,将FAdV-4的hexon-L1蛋白进行原核表达,免疫兔制备多克隆抗体,将多抗包被在检测(T)线,将羊抗兔IgG包被在质控(C)线,用胶体金标记的多抗作为示踪剂,制备胶体金免疫层析检测卡,用于检测FAdV-4抗原,并对其敏感性和特异性进行评价,用其检测临床样本并与PCR检测结果相比较。结果显示,制备的胶体金检测卡可检出FAdV-4含量为10^(2.094)^(5)EID_(50),FAdV-8、新城疫病毒、禽白血病病毒等均不出现特异性条带,对临床样本的检测与PCR检测的符合率达98%。建立的胶体金检测方法可用于FAdV-4感染的快速检测。

HPV L1壳蛋白与hTERC基因检测及联合分析对宫颈癌筛查的意义

目的探讨人乳头状瘤病毒(HPV)L1壳蛋白和人端粒酶RNA(hTERC)基因在宫颈脱落细胞中的表达及联合分析对宫颈癌筛查的意义。方法收集2008年1月至2009年5月北京大学深圳医院宫颈门诊就诊患者的宫颈脱落细胞标本309例,用免疫细胞化学法检测HPV L1壳蛋白的表达,荧光原位杂交(FISH)方法检测hTERC基因的表达。结果①随着组织学诊断级别的升高,HPV L1壳蛋白阳性表达率呈下降趋势,与宫颈病变的严重程度呈负相关(rs=-0.272,P<0.01);而hTERC阳性表达率呈增加趋势,与宫颈病变的严重程度呈正相关(rs=0.605,P<0.01)。②4种HPV L1/hTERC表达类型的构成与宫颈病变的级别有关。L1(-)/hTERC(+)表达类型在CIN2以上病变中的比例明显高于在CIN1中(P<0.01);L1(+)/hTERC(-)及L1(-)/hTERC(-)与宫颈病变的级别呈负相关(P<0.01),L1(-)/hTERC(+)与宫颈病变的级别呈正相关(P<0.01);从L1(-)/hTERC(-)、L1(+)/hTERC(-)、L1(+)/hTERC(+)到L1(-)/hTERC(+)在各级病变中的构成比有随宫颈病变级别增高而增加的趋势(P<0.01)。③HPVL1和hTERC联合检测的阴性预测值高于单用HPV L1或hTERC(P<0.05),但三者对宫颈癌筛查效率的差异无统计学意义(P>0.05)。结论 HPV L1壳蛋白和hTERC基因可作为早期诊断及预测宫颈病变的标志物。从L1(-)/hTERC(-)、L1(+)/hTERC(-)、L1(+)/hTERC(+)到L1(-)/hTERC(+),这种表达时序可能反映了宫颈病变的发展过程。

HPV L1壳蛋白在宫颈脱落细胞中的表达及临床意义

目的探讨人乳头状瘤病毒(HPV)L1壳蛋白在宫颈不同病变脱落细胞中的表达和临床意义。方法收集2008年1月至2009年5月到北京大学深圳医院宫颈门诊就诊患者的宫颈脱落细胞标本309例,其中正常或慢性宫颈炎33例、宫颈上皮内瘤变(CIN)Ⅰ级168例、CINⅡ/Ⅲ级84例和鳞状细胞癌(SCC)24例,用免疫细胞化学法检测HPV L1壳蛋白在宫颈脱落细胞中的表达。结果在正常宫颈或慢性宫颈炎、CINⅠ、CINⅡ/Ⅲ和SCC中,HPV L1壳蛋白阳性表达率分别为27.3%(9/33)、66.7%(112/168)、25.0%(21/84)、0%(0/24)。其中CINⅠ组、SCC组与正常或慢性宫颈炎组比较,CINⅠ组与CINⅡ/Ⅲ组比较,CINⅠ、CINⅡ/Ⅲ组与SCC组比较差异均有统计学意义(均P<0.01),随病变程度的加重,HPV L1壳蛋白阳性表达率呈下降的趋势。分别以30岁和40岁为界分组,不同年龄组间HPV L1壳蛋白的表达差异均无统计学意义(均P>0.05)。在高危型HPV DNA负荷量≥1 000 RLU/PC组HPV L1壳蛋白表达率为73.1%,与负荷量<1 000 RLU/PC的各组相比,其表达率明显增加(均P<0.05)。HPV L1壳蛋白检测CINⅡ/Ⅲ以上病变的敏感度、特异度、阳性预测值和阴性预测值分别为80.6%、60.2%、52.1%和85.2%。结论HPV L1壳蛋白在CIN和SCC中的阳性表达率随着病变程度加重呈下降趋势,有望成为预测宫颈癌前病变进展的生物学标志物。

原核表达系统中HPV16L1蛋白的表达与纯化

为了建立 HPV16 L1蛋白原核表达系统的纯化方法 ,纯化目的蛋白 ,我们构建了 p GEX4 T- HPV16 L1表达质粒。在大肠杆菌 BL2 1表达系统中表达 ,经过包涵体提取 ,8M尿素溶解 ,分级透析除去尿素 ,亲和层析进行提纯。结果显示 ,HPV16 L1蛋白在原核表达系统以不溶性包涵体形式存在 ,通过本方法可以获得纯化的 HPV16 L1蛋白 ,为 HPV16

PD-L1在乳腺癌及腋窝淋巴结中的表达及意义

目的检测人体乳腺癌组织及其腋窝淋巴结中PD L1蛋白的表达,进而探讨其在乳腺癌及其淋巴结中的表达情况与患者临床病理特征的关系。方法采用免疫组化染色法检测乳腺癌及其淋巴结中PD L1的表达。用统计软件分析其在乳腺癌及其淋巴结中的表达率与乳癌患者临床病理参数之间的关系。结果76例乳腺癌组织中癌细胞的细胞膜、细胞质及淋巴结转移灶中检测到PD L1的阳性表达,其中原发灶表达阳性率为25.0%,淋巴结转移灶表达阳性率21.4%。乳癌原发灶PD L1蛋白表达阳性率与患者淋巴结转移、TNM分期、ER及Her2的表达有关(P<0.05)。结论PD L1阳性表达的乳癌患者易发生淋巴结转移,预后较差,可作为评价乳癌患者预后的指标之一。

经基因优化的HPV16L1蛋白在毕赤酵母中的表达

目的利用毕赤酵母表达系统(Pichia pastoris)高效表达HPV16L1蛋白。方法按照Pichia pastoris密码子偏爱性合成HPV16L1基因,构建pAO819r-16L1表达载体,电转化至GS115菌株中,经MD板和不同浓度G418筛选,挑取高拷贝整合菌株,甲醇诱导目的蛋白的表达,用HPV16L1抗血清,经Western blot检测蛋白的特异性。结果重组质粒pAO819r-16L1在甲醇营养型酵母菌株中经甲醇诱导后可表达HPV16L1蛋白,在试管中的表达量超过10mg/ml,经Western blot验证,该蛋白可与抗血清特异结合,在相对分子质量55000附近出现目的条带,证明该蛋白确为HPV16L1蛋白。结论利用毕赤酵母表达系统可高效表达HPV16L1蛋白,为研制HPV疫苗奠定基础。