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Site-selective enzymatic chemistry for polymer conjugation to protein lysine residues: PEGylation of G-CSF at lysine-41

机译:聚合物与蛋白赖氨酸残基结合的定点酶化学:G-CSF在赖氨酸41处的聚乙二醇化

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摘要

Microbial transglutaminase (mTGase) is an enzyme that catalyzes site-specific protein derivatization at specific glutamines. mTGase-mediated conjugation with PEG-NH2 to granulocyte colony stimulating factor (G-CSF) yields a site selective mono-derivative conjugate involving Gln135. The same enzymatic reaction of mTGase, i.e. the transfer of the Gln acyl group to an amino donor, was investigated by reversing the substrates. A specific acyl donor PEG derivative was synthesized by coupling the Z-QG mTGase substrate to PEG. The mTGase-mediated conjugation of this PEG-ZQG in the presence of G-CSF generated a high-yield PEG-G-CSF conjugate in which the polymer was selectively coupled to Lys41 of the protein. The PEG-K41-G-CSF conjugate was compared with the PEG-Q135-G-CSF one obtained through mTGase conjugation of PEG-NH2 to Gln135. Biophysical characterization showed that the two positional isomers have similar behaviors, and pharmacokinetic studies in rats demonstrated that they have comparable half-life extensions. Overall, the study demonstrates that mTGase protein derivatization is linked to inherent advantages because it carries with it the possibility of targeting lysines or glutamines, in both cases with a high site-selective specificity.
机译:微生物转谷氨酰胺酶(mTGase)是一种催化特定谷氨酰胺处的位点特异性蛋白质衍生化的酶。 mTGase介导的PEG-NH2与粒细胞集落刺激因子(G-CSF)的缀合产生涉及Gln135的位点选择性单衍生物缀合物。通过反转底物,研究了mTGase的相同酶促反应,即Gln酰基向氨基供体的转移。通过将Z-QG mTGase底物与PEG偶联,可以合成特定的酰基供体PEG衍生物。在G-CSF的存在下,此PEG-ZQG的mTGase介导的偶联产生了高产率的PEG-G-CSF偶联物,其中聚合物被选择性偶联到蛋白质的Lys41。将PEG-K41-G-CSF缀合物与通过mTGase缀合PEG-NH 2至Gln135获得的PEG-Q135-G-CSF缀合物进行比较。生物物理特征表明这两个位置异构体具有相似的行为,并且在大鼠中的药代动力学研究表明它们具有相当的半衰期延长。总体而言,该研究表明,mTGase蛋白衍生化具有固有优势,因为在两种情况下,它都具有靶向赖氨酸或谷氨酰胺的可能性,而这两种情况都具有很高的位点选择性。

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