Optimization of Affinity Chromatography Based on Sepharose 4B- chitin for Rapid Purification of Urtica dioica Agglutinin.

IF 1.6 4区生物学 Q4 BIOTECHNOLOGY & APPLIED MICROBIOLOGY

Iranian Journal of Biotechnology Pub Date : 2023-07-01 DOI:10.30498/ijb.2023.339309.3364

Mohammadkazem Heydari, Abasalt Hosseinzadeh Colagar, Davood Sabour

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引用次数: 0

Abstract

Background: Today, numerous antimicrobial and anticancer properties have been reported for plant lectins due to their ability to bind to carbohydrates. The Urtica dioica agglutinin (UDA lectin) is a monomeric, small, and low molecular weight glycoprotein. It has attracted the attention of many researchers for identification, treatment, and other clinical purposes.

Objectives: The aim of this study is the optimization of the chitin affinity chromatography based on Sepharose 4B (CNBr-activated Sepharose 4B) for the rapid purification of UDA lectin from Urtica dioica rhizome.

Materials and methods: The chitin ligands were dissolved in 40% Trichloroacetic acid and attached to Sepharose 4B according to the Amersham-Biosciences instructions. The attachment of the ligand to the Sepharose 4B beads was investigated by Fourier transform infrared (FTIR) spectroscopy. An acidic crude extract of nettle rhizome passes from chromatographic columns in two sizes with dimensions: 24 x 0.51 cm and 8.44 x 0.86 cm. Quantity and quality of purified lectin were calculated by the Bradford microplate method: SDS-PAGE gel electrophoresis and human erythrocyte cell (RBC) hemagglutination, respectively.

Results: The analysis of FTIR spectrograms showed that major changes were observed in the fingerprint regions. Besides, due to the dissolution of Sepharose 4B and chitin in the aqueous phase, this difference was not significant in the Imine and Nitrile regions. On the other hand, the comparative results of purification chromatograms showed that increasing the column length causes a smaller half-width and increases the length of the purified peak. Also, it leads to high-quality purified UDA lectin, with a molecular weight of almost 12.5 kDa in gel electrophoresis. Hemagglutination activity on trypsinized red blood cells was displayed, and agglutination of purified UDA lectin started at least at 300 μg.mL^-1 concentration.

Conclusion: According to our findings, we suggested that dissolving chitin in the polar solvent of Trichloroacetic acid, using Sepharose 4B as the beads of a matrix, and increasing the column length might lead to a decrease in the half-width of the peak. These can increase the purity and concentration of purified UDA lectin, and speed up the purification process. These findings could be used by researchers to accelerate the purification of UDA lectin in other studies, dealing with drug delivery systems, ELISA techniques, and cell growth.

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优化基于 Sepharose 4B- chitin 的亲和层析技术，以快速纯化荨麻凝集素。

背景：如今，由于植物凝集素具有与碳水化合物结合的能力，因此有许多关于植物凝集素抗菌和抗癌特性的报道。荨麻凝集素（UDA凝集素）是一种单体、小分子和低分子量糖蛋白。它在鉴定、治疗和其他临床用途方面引起了许多研究人员的关注：本研究旨在优化基于 Sepharose 4B 的几丁质亲和层析（CNBr-activated Sepharose 4B），用于快速纯化荨麻根茎中的 UDA 凝集素：按照 Amersham-Biosciences 的说明，将几丁质配体溶解在 40% 的三氯乙酸中，并附着在 Sepharose 4B 上。配体附着到 Sepharose 4B 珠子上的情况通过傅立叶变换红外光谱（FTIR）进行了研究。荨麻根茎的酸性粗提取物从两种尺寸的色谱柱中通过：24 x 0.51 厘米和 8.44 x 0.86 厘米。纯化凝集素的数量和质量通过布拉德福德微孔板法进行计算：结果：傅立叶变换红外光谱图分析表明，指纹区域发生了重大变化。此外，由于 Sepharose 4B 和甲壳素溶于水相，在亚胺区和腈区的差异并不明显。另一方面，纯化色谱图的比较结果表明，增加色谱柱长度会使半宽变小，纯化峰的长度增加。此外，它还能纯化出高质量的 UDA 凝集素，凝胶电泳分子量接近 12.5 kDa。在胰蛋白酶化红细胞上显示出血凝活性，纯化的 UDA 凝集素至少在 300 μg.mL-1 浓度时开始凝集：结论：根据我们的研究结果，将甲壳素溶解在极性溶剂三氯乙酸中、使用 Sepharose 4B 作为基质珠、增加色谱柱长度可能会导致峰的半宽减小。这些方法可以提高纯化的 UDA 凝集素的纯度和浓度，加快纯化过程。这些发现可供研究人员在其他研究中加速 UDA 凝集素的纯化，包括药物输送系统、ELISA 技术和细胞生长。

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来源期刊

Iranian Journal of Biotechnology BIOTECHNOLOGY & APPLIED MICROBIOLOGY-

CiteScore

2.60

自引率

7.70%

发文量

期刊介绍： Iranian Journal of Biotechnology (IJB) is published quarterly by the National Institute of Genetic Engineering and Biotechnology. IJB publishes original scientific research papers in the broad area of Biotechnology such as, Agriculture, Animal and Marine Sciences, Basic Sciences, Bioinformatics, Biosafety and Bioethics, Environment, Industry and Mining and Medical Sciences.