Analysis of Major Royal Jelly Proteins Stability and Ligand Binding by Differential Scanning Fluorimetry

IF 0.3 Q4 FOOD SCIENCE & TECHNOLOGY
C. Mureșan, D. Dezmirean, Ramona Suharoschi, O. Pop, O. Borsai
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Abstract

Royal jelly (RJ) is produced by the hypopharingeal and mandibular glands of bees. Up to 90% of the RJ proteins are the major royal jelly proteins (MRJPs) that exhibit biological properties. Protein stability is of interest for biotechnology and can be explored by using differential scanning fluorimetry (DSF). We tested the stability by using a fluorescence dye (SYPRO® Orange,1:1000 dilution) in the presence of different ligands for MRJP1 and MRJP2 at 2 µM concentration. The fluorescence intensities (FI) were measured using the Real-Time PCR System and were fitted as a function of temperature according to the Boltzmann equation to determine the melting temperature (Tm) at which the amount of folded and unfolded protein is equal. In general, ligands stabilize the protein when binding to it and increase the Tm. Due to the increased starting fluorescence of the oligomeric MRJP1, the Tm values were only determined for monomeric MRJP1 and MRJP2. ATP, histamine, and thiamine were shown to determine an increase of Tm for the monomeric MRJP1 in 20 mM Tris-HCl, pH 7.4, 150 mM NaCl. For the ligand ATP, the minimum limit of binding starts at 1.5 mM concentration, for the ligand Histamine it starts at 0.6 mM concentration, while for the ligand Thiamine it starts at 3 mM concentration.
差动扫描荧光法分析蜂王浆主要蛋白的稳定性和配体结合
蜂王浆(RJ)是由蜜蜂的下咽腺和下颌腺产生的。高达90%的蜂王浆蛋白是主要的蜂王浆蛋白(MRJPs),具有生物学特性。蛋白质稳定性是生物技术研究的热点,可以通过差示扫描荧光法(DSF)来研究。我们使用荧光染料(SYPRO®Orange,1:1000稀释)在MRJP1和MRJP2的不同配体存在下,以2µM浓度测试其稳定性。荧光强度(FI)使用Real-Time PCR系统测量,并根据Boltzmann方程拟合温度的函数,以确定折叠和未折叠蛋白质数量相等的熔化温度(Tm)。一般来说,配体在与蛋白质结合时稳定蛋白质并增加Tm。由于低聚MRJP1的起始荧光增加,因此仅测定了MRJP1和MRJP2的Tm值。在20 mM Tris-HCl、pH 7.4、150 mM NaCl中,ATP、组胺和硫胺素决定了MRJP1单体Tm的增加。对于配体ATP,最小结合极限开始于1.5 mM浓度,对于配体组胺,它开始于0.6 mM浓度,而对于配体硫胺素,它开始于3 mM浓度。
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12
审稿时长
8 weeks
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