基于α-乳白蛋白基因序列的牛奶过敏原PCR检测

采用收集牛奶中脱落体细胞的方法提取牛奶DNA,针对牛奶过敏原蛋白α-乳白蛋白基因序列设计引物α-La-F/R,筛选适宜的实验条件,建立了检测牛奶过敏原的PCR方法.结果表明:PCR反应的最佳退火温度为56.5℃,引物浓度0.15μmol/L,循环数35,进一步实验表明该方法特异性良好,检测灵敏度可达到0.04ng DNA.将建立的PCR方法应用于10种食品的牛奶过敏原检测,实验结果与商品标示一致,表明该方法具有较高的准确性和可靠性,适用于实际商品中牛奶过敏原的检测.     

热加工方式对牛乳过敏原αs1-酪蛋白二级结构和抗原性的影响

为探究热加工方式对牛乳过敏原αs1-酪蛋白构象和抗原性的影响,利用间接竞争酶联免疫吸附测定方法、 免疫印迹方法分析不同加热条件下αs1-酪蛋白免疫原性的变化,进而通过8-苯胺-1-萘磺酸荧光探针和圆二色谱分 析其二级结构变化,初步揭示热处理调控过敏原αs1-酪蛋白抗原性的机制。结果表明：在80 ℃、60 min,90 ℃、 10 min,90 ℃、60 min条件下热处理后,αs1-酪蛋白中α-螺旋结构含量显著低于未加热αs1-酪蛋白,在70 ℃、 20 min,80 ℃、20 min,90 ℃、20 min条件下热处理后,αs1-酪蛋白中无规卷曲含量显著增加,70～100 ℃加热 20 min条件下表面荧光强度最强,其他温度-时间条件下二级结构含量变化不显著;αs1-酪蛋白构象的变化导致αs1-酪 蛋白的抗原性显著降低,间接竞争酶联免疫吸附测定显示,在70～100 ℃加热20 min条件下,αs1-酪蛋白的抗原残留 量均较高,而免疫印迹方法显示不同温度-时间条件下αs1-酪蛋白仍具有免疫反应特性,建议进一步通过动物实验揭 示热处理调控αs1-酪蛋白抗原性的机制。     

IgE reactivity to milk components in dogs with cutaneous adverse food reactions

We investigated the IgE reactivity to crude and purified milk antigens in the sera of 112 dogs with cutaneous adverse food reactions (CAFRs). Of the 112 dogs, 33 (29%) had specific IgE for crude milk antigens. In the dogs with milk-specific IgE, IgE reactivity to casein, bovine serum albumin (BSA), α-lactalbumin, β-lactoglobulin, and bovine IgG were 81%, 85%, 39%, 27%, and 35%, respectively. Casein and BSA may be important allergens in dogs with CAFRs. Some canine vaccines contain casein hydrolysate as a stabilizer and the pooled serum with anti-casein IgE showed IgE reactivity to the vaccines containing it. Information about IgE reactivity to casein in dogs with CAFRs could be useful for predicting adverse reactions to the vaccines including casein hydrolysate.     

辐照技术消减食物过敏原致敏性研究进展

食物过敏是当前威胁人类健康的重大食品安全问题之一。辐照技术可以消减食物过敏原,是一项颇具发展潜力的物理消敏技术。本文介绍了辐照消敏技术的特点、原理和发展历程,阐述了辐照消减动物源过敏食物牛乳、鸡蛋、虾、鱼等过敏原致敏性和植物源过敏食物花生、大豆、小麦、坚果等过敏原致敏性的研究进展,分析了辐照消减食物过敏原的效果和影响因素,探讨了辐照消敏技术的发展方向,以期为辐照消敏技术的研究和应用提供参考。     

Marker‐assisted backcrossing of a null allele of the α‐subunit of Soybean (Glycine max) β‐conglycinin with a Chinese soybean cultivar (a). The development of improved lines

The development of soybean varieties that lack the β‐conglycinin α‐subunit is an attractive goal because the β‐conglycinin α‐subunit negatively influences the nutrition and gelation of tofu and is a major allergen. To remove this undesirable allergen and simultaneously improve the seed nutritional value and food‐processing quality, marker‐assisted background selection (MABS) was used in backcross breeding to incorporate cgy‐2, a null phenotype version of the gene encoding the β‐conglycinin α‐subunit, from the donor line ‘RiB’ into the genetic background of the Chinese cultivar ‘Dongnong47’ (DN47), a popular high‐oil superfine seed soybean cultivar from Heilongjiang Province, China. In each F₂ (F₂, BC_nF₂) generation of the breeding programme, the offspring that carried the introgressed cgy‐2 were identified by sodium dodecyl sulphate–polyacrylamide gel electrophoresis and rescreened by MABS using simple sequence repeat markers to accelerate recurrent parent genome recovery. Of the 49 advanced backcrossing breeding lines (ABLs), the three best lines, ABL1, ABL2 and ABL3, were selected from the BC₁, BC₂ and BC₃ populations, respectively. The ABLs were evaluated for desirable agronomic characteristics, yield‐related traits, amino acid composition, free amino acid composition and tofu‐processing quality in the mature seeds. All of the ABLs lacked the α‐subunit but grew and reproduced normally without deleterious effects on physiological processes such as seed development and germination. The free amino acid content of ABL1 was significantly higher than that of ‘DN47’, with arginine (Arg) being particularly enriched. Compared to the recurrent parent ‘DN47’, the total protein content of the three ABLs was higher, the amino acid composition of the seed proteins was markedly modified and the yield and hardness of the tofu that was made from the ABLs were significantly increased. MABS combined with stringent phenotypic selection in a backcross breeding programme is a feasible strategy for the genetic engineering of seed protein components to produce allergenic subunit‐deficient variant alleles.     

应用生物信息学分析大米过敏原RAG1的B细胞表位(英文)

[目的]预测大米主要过敏原RAG1的二级结构及B细胞表位。[方法]从Expasy蛋白质数据库中获得编码大米过敏原RAG1的氨基酸序列并以此氨基酸序列为基础,通过DNAStarProtean软件,采用Gamier-Robson方案、Chou-Fasman方案和Karplus-Schulz方案预测RAG1的二级结构,用Kyte-Doolittle亲水性方案、Emini表面可及性方案、Jameson-Wolf抗原性指数方案综合预测RAG1的B细胞表位。[结果]对大米过敏原RAG1的二级结构和B细胞表位预测的结果表明,第33～44、119～129、155～163区段可能是B细胞的优势表位。[结论]本研究综合应用多方法多参数预测大米过敏原RAG1潜在的B细胞优势表位,为RAG1B细胞表位的进一步鉴定及其抗原性改造、表位疫苗设计等研究提供了理论依据。     

锯缘青蟹精氨酸激酶基因的克隆与表达

通过分子生物学方法,克隆得到锯缘青蟹（Scylla serrata）精氨酸激酶（Arginine Kinase,AK）开放阅读框基因序列.测序结果显示：该开放阅读框基因的序列长度为1 071 bp,编码356个氨基酸残基;该序列登录Genbank（GQ：851626）,序列比对结果显示,锯缘青蟹精氨酸激酶与凡纳滨对虾（Litopenaeus vannamei）精氨酸激酶的氨基酸序列同源性高达94%,与岸蟹（Carcinus maenas）、中华绒鳌蟹（Eriocheir sinensis）等甲壳类动物的精氨酸激酶也有较高的同源性,均高于90%;将克隆得到的锯缘青蟹精氨酸激酶基因与pGEX-4T-3载体连接,转化大肠杆菌BL21,经IPTG诱导得到分子质量为65 ku的融合表达蛋白（GST-AK）,经兔抗锯缘青蟹精氨酸激酶多克隆抗体的免疫印迹分析证实,GST-AK具有抗原性.