Thermal-aggregation suppression of proteins by a structured PEG analogue: Importance of denaturation temperature for effective aggregation suppression |
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| Affiliation: | 1. Charles University, Faculty of Mathematics and Physics, Dept. of Condensed Matter Physics, Prague, Czech Republic;2. Stockholm University, Dept. of Materials and Environmental Chemistry, SE-106 91 Stockholm, Sweden;3. Charles University, Faculty of Mathematics and Physics, Dept. of Physics of Materials, Prague, Czech Republic;4. Institute of Macromolecular Chemistry, Academy of Sciences of the Czech Republic, Prague, Czech Republic |
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| Abstract: | Development of protein stabilizing reagents, that suppress aggregation and assist refolding, is an important issue in biochemical technology related with the synthesis and preservation of therapeutic or other functional proteins. In the precedent research, we have developed a structured poly(ethylene glycol) (PEG) analogue with triangular geometry, which turns into a dehydrated state above ca. 60 °C. Focusing on this rather lower dehydration temperature than that of conventional linear PEGs, a capability of the triangle-PEG to stabilize proteins under thermal stimuli was studied for citrate synthase, carbonic anhydrase, lysozyme and phospholipase. Variable temperature high-tension voltage and circular dichroism spectroscopic studies on the mixtures of these proteins and the triangle-PEG showed that the triangle-PEG stabilizes carbonic anhydrase, lysozyme and phospholipase that exhibit denaturation temperatures higher than 60 °C, while substantially no stabilization was observed for citrate synthase that denatures below 60 °C. Hence, the dehydrated triangle-PEG likely interacts with partially unfolded proteins through the hydrophobic interaction to suppress protein aggregation. |
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| Keywords: | Poly(ethylene glycol) Aggregation Circular dichroism spectroscopy High-tension voltage analysis Protein denaturation Refolding |
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