首页> 外文OA文献 >Cloning and expression of biologically active Plantago lanceolata pollen allergen Pla l 1 in the yeast Pichia pastoris.
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Cloning and expression of biologically active Plantago lanceolata pollen allergen Pla l 1 in the yeast Pichia pastoris.

机译:具有生物活性的车前草花粉过敏原Pla 1在酵母毕赤酵母中的克隆和表达。

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摘要

The glycoprotein Pla l 1 is the major allergen from English plantain (Plantago lanceolata) pollen, which is a common cause of pollinosis in temperate areas. Three complete cDNAs for Pla l 1 isoforms were isolated by PCR using specific 3' and 5' primers. All three Pla l 1 cDNAs code for a 25-residue leader peptide and a 131-residue mature protein that contains two polymorphic positions, an N-glycosylation site at position 107 and six cysteine residues involved in three disulphide bridges. The allergen variant Pla l 1.0101 was produced in Pichia pastoris at a yield of 20 mg per litre of culture as a mixture of non-glycosylated (17 kDa), glycosylated (23 kDa) and dimeric (32-39 kDa) forms. Recombinant Pla l 1 (rPla l 1) was purified by affinity chromatography with an anti-natural Pla l 1 (anti-nPla l 1) monoclonal antibody, and its molecular and immunological properties were compared with the natural allergen by CD spectroscopic analysis, enzymic deglycosylation, lectin-binding assay, immunodetection and ELISA-inhibition assays using sera from plantain-allergic patients. The recombinant allergen is properly folded, as deduced from CD spectra, and the immunodominant allergenic epitopes of the natural allergen are preserved in rPla l 1. These results allow us to conclude that P. pastoris is a convenient system for the efficient production of biologically active rPla l 1, which could have a potential use for clinical purposes. Furthermore, a sequence similarity of Pla l 1 to the major allergen from the olive tree pollen, Ole e 1, is revealed in this work, and the allergenic cross-reactivity between both allergens has been studied.
机译:糖蛋白Pla 1是来自英国车前草(Plantago lanceolata)花粉的主要变应原,这是温带地区花粉病的常见原因。使用特定的3'和5'引物通过PCR分离了Pla 1同工型的三个完整cDNA。所有三个Pla 1 cDNA编码一个25个残基的前导肽和一个131个残基的成熟蛋白,该蛋白包含两个多态性位置,一个位于107位的N-糖基化位点和六个涉及三个二硫键的半胱氨酸残基。变应原变体Pla 111.101在毕赤酵母中以每升培养物20mg的产量产生,其为非糖基化(17kDa),糖基化(23kDa)和二聚体(32-39kDa)形式的混合物。用抗天然Pl 1 1(抗nPla 1 1)单克隆抗体通过亲和层析纯化重组Pla 1 1(rPla 1 1),并通过CD光谱分析,酶促法将其分子和免疫学性质与天然过敏原进行比较。用车前草过敏患者的血清进行脱糖基化,凝集素结合测定,免疫检测和ELISA抑制测定。根据CD光谱推断,重组过敏原经过适当折叠,天然过敏原的免疫优势致敏表位保存在rPla 1中。这些结果使我们得出结论,巴斯德毕赤酵母是高效生产具有生物活性的方便系统。 rPla 1,可能具有临床用途。此外,这项工作揭示了Pl 1 1与来自橄榄树花粉的主要过敏原的序列相似性,并且研究了两种过敏原之间的过敏原交叉反应性。

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