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用于捕获低分子量蛋白质和肽的核壳型硅纳米粒子的新合成方法。

Novel Synthesis of Core-Shell Silica Nanoparticles for the Capture of Low Molecular Weight Proteins and Peptides.

机构信息

Centro de Investigación en Alimentación y Desarrollo A.C. Carretera a la Victoria km 0.6 C.P. 83304, Hermosillo 83304, Sonora, Mexico.

Universidad de Sonora. Blvd. Luis Encinas y Rosales S/N, Col. Centro, Hermosillo 83000, Sonora, Mexico.

出版信息

Molecules. 2017 Oct 12;22(10):1712. doi: 10.3390/molecules22101712.

Abstract

Silica nanoparticles were functionalized with immobilized molecular bait, Cibacron Blue, and a porous polymeric bis-acrylamide shell. These nanoparticles represent a new alternative to capture low molecular weight (LMW) proteins/peptides, that might be potential biomarkers. Functionalized core-shell silica nanoparticles (FCSNP) presented a size distribution of 243.9 ± 11.6 nm and an estimated surface charge of -38.1 ± 0.9 mV. The successful attachment of compounds at every stage of synthesis was evidenced by ATR-FTIR. The capture of model peptides was determined by mass spectrometry, indicating that only the peptide with a long sequence of hydrophobic amino acids (alpha zein 34-mer) interacted with the molecular bait. FCSNP excluded the high molecular weight protein (HMW), BSA, and captured LMW proteins (myoglobin and aprotinin), as evidenced by SDS-PAGE. Functionalization of nanoparticles with Cibacron Blue was crucial to capture these molecules. FCSNP were stable after twelve months of storage and maintained a capacity of 3.1-3.4 µg/mg.

摘要

硅胶纳米颗粒通过固定化分子诱饵 Cibacron Blue 和多孔聚合物双丙烯酰胺壳进行功能化。这些纳米颗粒为捕获低分子量(LMW)蛋白质/肽提供了一种新的替代方法,这些蛋白质/肽可能是潜在的生物标志物。功能化核壳硅胶纳米颗粒(FCSNP)的粒径分布为 243.9±11.6nm,表面电荷估计为-38.1±0.9mV。通过衰减全反射傅里叶变换红外光谱(ATR-FTIR)证实了在合成的每个阶段化合物的成功附着。通过质谱法确定了模型肽的捕获,表明只有具有长序列疏水性氨基酸(α玉米醇溶蛋白 34 肽)的肽与分子诱饵相互作用。FCSNP 排除了高分子量蛋白质(BSA)和捕获的低分子量蛋白质(肌红蛋白和抑肽酶),这一点通过 SDS-PAGE 得到了证实。用 Cibacron Blue 对纳米颗粒进行功能化对于捕获这些分子至关重要。FCSNP 在储存 12 个月后仍然稳定,保持 3.1-3.4μg/mg 的容量。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/0e1a/6151791/e82832427efe/molecules-22-01712-g001.jpg

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