Characterization of physicochemical and immunogenic properties of allergenic proteins altered by food processing:a review

Food allergens are mainly naturally-occurring proteins with immunoglobulin E(IgE)-binding epitopes.Understanding the structural and immunogenic characteristics of allergenic proteins is essential in assessing whether and how food processing techniques reduce allergenicity.We here discuss the impacts of food processing technologies on the modification of physicochemical,structural,and immunogenic properties of allergenic proteins.Detection techniques for characterizing changes in these properties of food allergens are summarized.Food processing helps to reduce allergenicity by aggregating or denaturing proteins,which masks,modifies,or destroys antigenic epitopes,whereas,it cannot eliminate allergenicity completely,and sometimes even improves allergenicity by exposing new epitopes.Moreover,most food processing techniques have been tested on purified food allergens rather than food products due to potential interference of other food components.We provide guidance for further development of processing operations that can decrease the allergenicity of allergenic food proteins without negatively impacting the nutritional profile.

Characterization of ST13 Protein Expression in Human Colorectal Cancer Tissues

Objective: To characterize the expression of ST13 protein in human tissuesfor investigation of the function of colorectal cancer related gene ST13. Methods: ST13 ORF wascloned and over-expressed in E.coli. The recombinant ST13 protein was purified by affinitychromatography. ST13 monoclonal antibodies were generated and affinity purified with the recombinantprotein. Immunoblot and immunohistochemical staining were employed to analyze ST13 proteinexpression in human tissues. Results: The expression and purification of the recombinant ST13protein were confirmed by SDS-PAGE. The protein yield reached about 2.5 mg/L of induced bacterialculture with a purity of 91.3%. Three strains of hybridoma were obtained with antibody titers from10~4 to 10~5 in ascites fluids and with high specificity for ST13 protein. Immunoblot showed thatthe apparent Mr of ST13 protein in SW480 cells and human tissues estimated by SDS-PAGE mobility wasapproximately 50 000, which was about 10 000 larger than the 41 324 calculated, but theglycosylation of the protein was excluded. Computer modeling revealed the protein to be ahydrophilic molecule. Immunohistochemical staining showed that ST13 protein was evenly distributedin cytoplasm and expressed in colon, stomach, liver, and other epithelial cells. Differences in thestaining intensity of the protein were observed between normal and cancer tissues as well as amongdifferent normal or carcinoma tissues. Conclusion: ST13 protein is a cytoplasmic molecule with anapparent Mr of 50 000. The protein is expressed in colorectal and other epithelial tissues. Theexpression level of the protein is down-regulated in colorectal cancer and varies among differentnormal and/or carcinoma tissues. Comparison of cDNA sequences and protein characteristics indicatesthat ST13 protein and hsp70-interacting protein (Hip) are same proteins, raising the possibilitythat ST13 protein is involved in the development of colorectal cancer through Hsp70 molecularchaperone machinery.

Purification and Characterization of Cyclic AMP-Binding Protein from Ganoderma lucidum

Cyclic AMP-binding protein was purified 30 fold from the mycelia of Ganoderma lucidum by the methods of ammonium sulfate precipitation, DEAE-cellulose, phospho-cellulose ion exchange chromatography and Sephacryl S-100 gel filtration. The molecular mass of the purified protein is 34.5 kDa and 17 kDa by Sephacryl S-100 gel filtration and SDS-ployacrylamide gel electrophoresis, respectively. From these results it is suggested that the protein has a homometric dimmer structure. The pI of the purified protein is pH 8.2 by native isoelectric focusing gel. The half-life of the protein activity in 10% glycerol at 4 ℃ is 7 d in crude extract, but its half-life is only 3 d under purifying conditions. The optimal conditions of the protein activity are at 1 ℃ and pH 7.5. Its activity is increased 6 times by 1 mmol/L Zn^(2+) and is slightly inhibited by cGMP, Cu^(2+) and Mn^(2+).

Expression Characterization and Preparation of Human Amyloid Precursor Protein in Escherichia coli

To analyze whether expressed amyloid precursor protein（APP） existed in hydrophilic（cytoplasmid） or hydrophobic（lipid bilayer） environment in E. coli and to obtain intact APP for study on its function, we investigated the expression characterization and preparation of the three intact isoforms APP770, APP751, and APP695 in E. coll. The results show that these expressed APPs existed both in hydrophilic cytoplasm region as inclusion bodies and hydrophobic membrane region as membrane-bound state in E. coll. APPs in inclusion bodies were purified on an NTA-Ni^2＋ agarose column after dissolving in the urea buffer and APPs in membrane-bound state were obtained by ultracentrifugation. The activity analysis indicates that APP770 and APP751 exhibited strong trypsin-inhibitory activity like the natural ones. These results indicate that E. coli cells can be used as host cells for the expression of human integral membrane protein like APP in either soluble or membrane-bound state unless the interest protein undergone post-translational modification is required.

Characterization of Influenza H5N1 Nucleocapsid Protein for Potential Vaccine Design

Avian influenza, subtype H5N1, causes occasional but serious infections in humans and efforts to produce vaccines against this strain continue. Current influenza vaccines are prophylactic and utilize the two major antigens, hemagglutinin and neuraminidase. Nucleocapsid protein (NP) is an attractive alternative antigen because it is highly conserved across all influenza strains, has been shown to increase the rate of viral clearance, and potential therapeutic vaccines would elicit cytotoxic T lymphocyte responses in an infected person. The NP antigen from H5N1 was characterized using a variety of physico-chemical methods to gain insights into both the biological and physical properties of the antigen which are important from a regulatory viewpoint when considering therapeutic vaccines. Results obtained to date show that NP is relatively unstable and indicate that the conformation of the H5N1 NP antigen is highly dependent upon purification procedure, buffer conditions, pH and the presence or absence of RNA. These factors will need to be clearly defined and taken into consideration when manufacturing and regulating NP vaccine preparations.

Molecular Cloning,Expression,and Characterization of an Adenylyl Cyclase-associated Protein from Gossypium arboreum Fuzzless Mutant

CAP,an adenylyl cyclase-associated protein,is predicted to be involved in cytoskeletal organization and signal transduction.Recently,we found that CAP may play an important role in fuzz-like fiber cell initiation in cotton.For the further research,we isolated two CAP homologues from wild

Cloning and Characterization of a Novel cDNA Encoding Late Embryogenesis-Abundant Protein 5 Like (LEA-5) Gene from Cara Cara Navel Orange Fruit (Citrus sinensis Osbeck)

LEA5 gene was postulated related with both stress and hormone responses. In an attempt to find genes exclusively expressed during fruit ripening of Cara Cara navel orange, a novel cDNA clone encoding late embryogenesis-abundant protein 5 like gene （CitLEA5-1） was obtained. It was 582 bp in length, containing 97 deduced amino acids. Compared with the stress-induced LEA5 from leaves of Citrus sinensis, CitLEA5-1 had a shorter 3′ untranslated region （UTR）. Semi-quantitative RT-PCR analysis revealed that CitLEA5-1 was transcriptional regulated during fruit ripening of Cara Cara navel orange.

Expression and Characterization of Catalytic Domain of T Cell Protein Tyrosine Phosphatase(ΔTC-PTP)——Immunohistochemical Study of ΔTC-PTP Expression in Non-small Cell Lung Carcinomas

This study objective was to express and characterize the catalytic domain of the human T cell protein tyrosine phosphatase（△TC-PTP） and to study immunohistochemically the expression of △TC-PTP in human non-small cell lung cancers. △TC-PTP gene was PCR amplified with the cDNA of human TC-PTP as template, and cloned into the pT7 expression vector. The recombinant pT7-△TC-PTP was expressed in E. coli Rosetta （ DE3 ） host cells and puri- fied. The enzymatic characteristics of △TC-PTP including enzyme activity and kinetics assay were measured. The antiserum was prepared by immunizing rabbit with the purified recombinant △TC-PTP. Rabbit polyclonal antibody against △TC-PTP was purified by PVDF immobilized antigen affinity chromatography. Immunohistochemical staining of lung cancer tissues was performed with antibody against △TC-PTP protein. △TC-PTP gene was correctly cloned, expressed, and purified. The recombinant △TC-PTP had a highly catalytic activity of PTPase. Squamous cell lung carcinoma showed a significantly higher expression rate of △TC-PTP （76. 92%, 10/13 ） than adenocarcinoma （57.14%, 4/7） and normal lung tissue（20%, 1/5 ）. This study represents the first demonstration that △TC-PTP is highly expressed in human squamous cell lung carcinomas. In addition, this study provides an important basis for further studying the biological function of TC-PTP and its relationship with lung carcinomas and other diseases.

Cloning, Characterization and Bioinformatic Analysis of the Gene Encoding the Larval Serum Protein 2 in Diapause of the Onion Maggot, Delia Antiqua

The full-length cDNA encoding Larval serum protein 2 (LSp-2) in the onion maggot,Delia antiqua, was cloned and sequenced by rapid ampli?cation of cDNA ends methods. The result showed that the cDNA was 2203 bp long and the open reading frame (ORF) of 2106 bp encoded 701 amino acid with a calculated molecular weight of 80.5 kDa and an isoelectric point of 5.87. The onion maggot LSp-2 shows highest homology (83%) to that ofCalliphora vicinaat amino acid level. Its signal peptides, domains and structures were predicted and analyzed by using bioinformatic methods. The amino acid sequence of LSP-2 suggests that it would be a typical hexamerin.

超声波、微波预处理对核桃粕蛋白肽钙螯合能力、结构及稳定性的影响

本研究基于超声波、微波预处理核桃粕蛋白肽及CaCl_(2)的混合物制备核桃粕蛋白肽钙螯合物。分析不同处理对核桃粕蛋白肽钙螯合率、结构变化及稳定性的影响。结果表明,相较未处理的核桃粕蛋白肽钙螯合物(WPP-Ca),超声波处理核桃粕蛋白肽钙螯合物(UP-WPP-Ca)和微波处理核桃粕蛋白肽钙螯合物(MP-WPP-Ca)的螯合率均有所提升,超声波和微波处理有效提高了肽钙螯合能力。基于紫外-可见吸收光谱、傅里叶变换红外光谱分析,发现超声波、微波主要是影响了核桃粕蛋白肽的氨基、羰基、羧基、酰胺键及羧酸盐基团等钙离子结合位点;X射线衍射结果表明超声波、微波处理改变了核桃粕蛋白肽的分子排列进而使核桃粕蛋白肽钙螯合物的结构更有序;荧光光谱结果表明超声波、微波处理促进了芳香族氨基酸与钙离子的螯合。此外,UP-WPP-Ca和MP-WPP-Ca在不同pH值、温度和胃肠道消化中表现出良好的稳定性。总之,超声波、微波预处理后进行的核桃粕蛋白肽钙螯合反应可提高其钙离子螯合能力和稳定性,结果对核桃粕蛋白肽钙螯合物的加工生产及补钙产品的开发具有一定的指导意义。

尿素-乙二醛树脂改性大豆蛋白胶黏剂的制备及性能研究

以尿素-乙二醛(UG)树脂和大豆分离蛋白(SPI)为主要原料制备大豆蛋白胶(SUG),并对其固体含量、黏度、表面张力系数、接触角及胶合性能进行测试;利用XPS、FT-IR和^(13)C NMR对合成的SUG的结构进行表征;采用DSC及DMA对SUG的固化性能进行测定。研究结果表明:改性后大豆蛋白胶的固体含量、黏度、表面张力系数及接触角随着SPI添加量的增加而增大,其中黏度的变化最显著;合成大豆蛋白胶中主要含有C—C、C—O—C、C=O、C=N、C=O等官能团;结合^(13)C NMR及FT-IR分析结果,可以得出UG树脂与SPI二者之间产生了交联;当SPI用量为30 g,UG树脂用量为50 g时,制备的大豆蛋白基胶黏剂性能较佳且固化后储能模量较大,为4082 MPa,在160和180℃热压温度下制备的胶合板冷水24 h湿强度分别为1.23和1.48 MPa,热水3 h湿强度分别为1.05和1.22 MPa,远大于国家标准GB/T 9846—2015对II类胶合板的要求,且具备一定的耐沸水性能。

小麦水解蛋白的结构表征及其体外稳定性研究

对小麦水解蛋白进行了结构表征,研究了不同加工条件对小麦水解蛋白稳定性的影响。结果显示:小麦水解蛋白的α-螺旋、平行式β-折叠、反平行式β-折叠、β-转角和无规则卷曲含量分别为18.46%±0.29%、6.85%±0.21%、37.34%±0.50%、18.30%±0.30%、19.05%±0.29%,β-折叠为小麦水解蛋白的主要二级结构,小麦水解蛋白呈球状,表面有小孔和不规则的褶皱。热处理对小麦水解蛋白的重均分子量和二级结构无明显影响;在不同pH条件下小麦水解蛋白的二级结构较稳定,但相对于酸性环境,在碱性环境下其稳定性较差;体外模拟消化试验表明小麦水解蛋白体外消化稳定性较差。

亚麻籽分离蛋白结构表征及其性能分析

为实现亚麻籽饼粕中分离蛋白的综合加工利用,该文以冷榨亚麻籽饼粕为原料,对其进行脱胶脱脂处理,采用超声辅助水提法分别提取亚麻籽分离蛋白和脱胶脱脂亚麻籽分离蛋白,并对理化性质、结构及功能特性进行分析比较。结果表明,冷榨亚麻籽饼粕和脱胶脱脂亚麻籽饼粕中蛋白质质量分数分别为37.52%±0.04%、37.47%±0.02%。采用十二烷基硫酸钠-聚丙烯酰胺凝胶电泳测定亚麻籽分离蛋白和脱胶脱脂亚麻籽分离蛋白的分子质量,显示10~55 kDa之间有明显谱带,其中水溶性低分子质量的白蛋白(10、14、15及17 kDa)和盐溶性高分子质量的球蛋白(30、33、35、40、45及55 kDa)谱带最为明显。氨基酸的种类各检测到17种,含有丰富的必需氨基酸和非必需氨基酸。傅里叶变换红外光谱测定的2种蛋白质的二级结构稳定性一般;由扫描电镜和X-射线衍射可知亚麻籽分离蛋白比脱胶脱脂亚麻籽分离蛋白的微观孔隙率低,结构中都较缺乏结晶度或有序排列。2种蛋白的两亲性与大豆分离蛋白相比,亲水/油特性突出,亲油性是大豆分离蛋白的2倍多。对不同pH(2~11)和盐离子浓度(0~1.25 mol/L)下溶解度、起泡性、泡沫稳定性、乳化活性及乳化稳定性的测定显示,两者具有良好的碱溶性,脱胶脱脂亚麻籽分离蛋白的起泡性、乳化活性及乳化稳定性均优于亚麻籽分离蛋白,而泡沫稳定性恰好相反,该研究结果有利于拓宽2种分离蛋白在健康食品领域中的应用前景,为食品中的应用提供有益参考和数据支撑。

引起典型PDNS的PCV-2病原分子特征分析

为了了解引起贵州省贵定县某猪场育肥猪群出现的典型猪皮炎肾病综合征(PDNS)的PCV-2的分子特征,试验首先对采自该猪场患病猪血清进行PCR扩增和克隆测序,然后采用多种分子生物学软件及网站对PCV-2的基因型、基因结构、推导蛋白等进行研究。结果表明:PCR扩增得到大小为1767 bp的条带,与GenBank中CZ246毒株序列(登录号为MZ995482)的相似性最高,将获得的毒株命名为PCV-2 GZGD2022。PCV-2 GZGD2022株为PCV-2d基因型,与PCV-2d参考株NLControl4(登录号为AY484410)相比,含10个开放阅读框(ORF),缺失ORF8,其ORF5终止密码子提前,大小仅为21 bp。该毒株在基因组第1042位有1个碱基T的缺失,但导致Cap蛋白C末端延伸的是脯氨酸(P)而非赖氨酸(K)。与疫苗株(LG株、DBN-SX07-2株、ZJ株、SH株)相比,在Cap蛋白的抗原表位区有7个特异性突变点(F53I、R59K、A68N、T134N、A190T、A68N、T134N)。上述疫苗株之间磷酸化位点的差异主要集中在Cap蛋白上,在88 aa处多了1个丝氨酸磷酸化位点,在47 aa、134 aa、149 aa处少了1个苏氨酸磷酸化位点,在55 aa和218 aa处少了1个酪氨酸磷酸化位点。Rep蛋白有3个N糖基化位点(23NPS25、256NQT258和286NAT288),Cap蛋白有1个N糖基化位点(143NYS145)。Rep、Cap蛋白为混合型蛋白。此外,Rep、Cap蛋白有一些特殊功能结构域,如前者的PH-LIKE、NACHT等结构域和后者的乙酰化修饰位点(1MTYPR6)与核定位信号(NLS)。说明引起贵州省贵定县某猪场猪群出现典型PDNS的致病株为PCV-2d基因型,该毒株缺失ORF8,编码蛋白的氨基酸、抗原表位和磷酸化位点的改变可能是导致其毒力较强、引起典型PDNS的原因。

富硒小米蛋白的理化性质、功能特性及结构研究

该文以普通小米蛋白(common millet protein,MP)为对照,采用十二烷基硫酸钠聚丙烯酰胺凝胶电泳(sodium dodecyl sulfate polyacrylamide gel electrophoresis,SDS-PAGE)、傅里叶红外光谱(Fourier infrared spectroscopy,FT-IR)、扫描电镜(scanning electron microscopy,SEM)等方法并测定溶解度(solubility,PS)、持水性(water holding capacity,WA)、乳化性(emulsification capability,EC)等指标对富硒小米蛋白(selenium-rich millet protein,SMP)的理化性质、功能特性及结构进行分析。结果表明,MP与SMP的硒含量分别为0.08、0.63 mg/kg;MP与SMP的必需氨基酸(essential amino acid,EAA)含量分别占总氨基酸含量的51.101%、53.529%;EAA与非必需氨基酸(non-essential amino acids,NEAA)的比值为1.045、1.152;2种小米蛋白分子质量均分布在10~70.2 kDa;随着pH升高,小米蛋白的PS、WA、起泡性(froth capability,FC)、起泡稳定性(froth stability,FS)、EC均呈现先下降后上升趋势,而乳化稳定性(emulsion stability,ES)正好相反;随着温度升高,小米蛋白的PS、WA、持油性(oil-holding property,FA)、FC、FS、EC、ES均呈现先上升后下降趋势(P<0.05);SEM结果显示MP表面有不规则凸起,而SMP表面光滑平整;FT-IR显示2种小米蛋白峰型一致,SMP位置略有后移,同时SMP的α-螺旋、β-折叠、β-转角含量较MP分别高出5.532、2.885、5.506个百分点,无规则卷曲含量则低于MP,说明SMP的结构有序性优于MP。该研究结果为SMP产品的开发利用提供重要理论依据。

Claudin18.2分子特征概述及其作为治疗靶点在胃癌中的研究进展

作为紧密连接蛋白(Claudin,CLDN)家族成员之一,Claudin18.2(CLDN18.2)在正常情况下仅在正常胃黏膜上皮细胞中表达,以维持细胞正常功能。但在异常情况下,CLDN18.2在包括胃癌在内的多种恶性肿瘤中呈高表达状态,使其成为治疗前景非常高的新靶点。目前,靶向CLDN18.2的抗肿瘤新药研发如火如荼,药物类型和治疗策略呈现多样化。本文旨在概述CLDN18.2的分子特征,并对胃癌中靶向CLDN18.2的新药/新技术研发现状进行梳理,包括单克隆抗体、双特异性抗体、抗体药物偶联物、嵌合抗原受体T细胞免疫疗法、纳米抗体等。

普通烟草β-半乳糖苷酶基因(NtBGAL)的生信分析及其在不同组织及原核诱导的表达

【目的】探明普通烟草β-半乳糖苷酶基因NtBGAL的表达模式与蛋白特征,为后期创制烟草多用途利用的底盘材料提供依据。【方法】通过比对普通烟草K326基因序列与本氏烟草NbBGAL1基因的同源性,以K326的cDNA为模板经PCR技术克隆获得NtBGAL基因,随后利用生信工具软件分析其基因结构及蛋白理化性质,并采用qRT-PCR检测该基因在烟草不同组织部位(根、茎、叶和花)的表达模式,最后开展原核诱导表达、蛋白纯化及蛋白表征研究。【结果】克隆获得烟草NtBGAL基因,其与本氏烟草NbBGAL1基因同源性最高,二者具有相同的结构域(Motif);该基因定位于9号染色体上,含有18个内含子,mRNA长度为6649 bp,CDS长度为2541 bp,编码846个氨基酸,翻译的β-半乳糖苷酶属于GH35家族,NtBGAL蛋白的分子量为92.44 kDa,理论等电点(pI)为6.8,GRAVY为-0.222,定位于细胞壁。该基因在普通烟草不同组织部位的表达量为花>叶>茎>根,差异显著。在37℃下进行原核诱导,NtBGAL蛋白有明显表达;采用包涵体纯化方法获得较高纯度的NtBGAL蛋白。NtBGAL蛋白酶促反应最适温度为30~40℃,最适pH为4.0~6.5,Mn^(2+)浓度为0.05~0.15 mmol/L时对NtBGAL酶活性有增强作用。【结论】研究明确NtBGAL基因的组织表达模式及蛋白表征,为进一步通过改造NtBGAL基因,利用普通烟草生产人源化糖蛋白奠定基础。

牦牛乳酪蛋白琥珀酸铁的制备及其结构表征

为了充分利用牦牛乳资源,以牦牛乳酪蛋白为原料,采用响应面分析法确定牦牛乳酪蛋白的最佳酰化条件,制备高质量、生物利用率好的蛋白琥珀酸铁制品;采用傅里叶红外光谱、粒径分布、扫描电子显微镜、氨基酸组成、体外模拟消化等手段对制品进行结构表征。结果表明:牦牛乳酪蛋白最佳酰化工艺参数为:酪蛋白与丁二酸酐质量比2∶1,丁二酸酐分5次加入,pH 9,反应温度48℃,反应时间50 min,在此条件下酰化率达到93.27%,含铁量8%,螯合率93.03%。傅里叶红外光谱测定结果显示:蛋白琥珀酸铁与酪蛋白的吸收峰存在差异,酰化蛋白中铁离子与羧基、氨基形成配位键。用激光粒度分布仪测得蛋白琥珀酸铁粒径更大,证实形成螯合物。扫描电子显微镜分析表明样品表面光滑,结构紧密。通过测定蛋白琥珀酸铁的蛋白含量及氨基酸组成,得出蛋白琥珀酸铁较酪蛋白蛋白质损失28.12%。酪蛋白与蛋白琥珀酸铁中Glu、Asp和Pro含量较高,其中Glu和Asp是形成螯合物的关键氨基酸,且生物利用率优于无机盐。本研究结果可为蛋白琥珀酸铁制备以及结构表征提供参考。