Immobilised-enzyme microreactors for the identification and synthesis of conjugated drug metabolites

被引:2
|
作者
Doyle, Bradley [1 ]
Madden, Leigh A. [2 ]
Pamme, Nicole [1 ,3 ]
Jones, Huw S. [4 ]
机构
[1] Univ Hull, Sch Nat Sci, Kingston Upon Hull HU6 7RX, N Humberside, England
[2] Univ Hull, Ctr Biomed, Kingston Upon Hull HU6 7RX, N Humberside, England
[3] Stockholm Univ, Dept Mat & Environm Chem, S-10691 Stockholm, Sweden
[4] Univ Bradford, Inst Canc Therapeut, Bradford BD7 1DP, W Yorkshire, England
关键词
QUANTIFICATION; INHIBITION; DISCOVERY; REACTOR; CELLS;
D O I
10.1039/d3ra03742h
中图分类号
O6 [化学];
学科分类号
0703 ;
摘要
The study of naturally circulating drug metabolites has been a focus of interest, since these metabolites may have different therapeutic and toxicological effects compared to the parent drug. The synthesis of metabolites outside of the human body is vital in order to conduct studies into the pharmacological activities of drugs and bioactive compounds. Current synthesis methods require significant purification and separation efforts or do not provide sufficient quantities for use in pharmacology experiments. Thus, there is a need for simple methods yielding high conversions whilst bypassing the requirement for a separation. Here we have developed and optimised flow chemistry methods in glass microfluidic reactors utilising surface-immobilised enzymes for sulfonation (SULT1a1) and glucuronidation (UGT1a1). Conversion occurs in flow, the precursor and co-factor are pumped through the device, react with the immobilised enzymes and the product is then simply collected at the outlet with no separation from a complex biological matrix required. Conversion only occurred when both the correct co-factor and enzyme were present within the microfluidic system. Yields of 0.97 & PLUSMN; 0.26 & mu;g were obtained from the conversion of resorufin into resorufin sulfate over 2 h with the SULT1a1 enzyme and 0.47 & mu;g of resorufin glucuronide over 4 h for UGT1a1. This was demonstrated to be significantly more than static test tube reactions at 0.22 & mu;g (SULT1a1) and 0.19 & mu;g (UGT1a1) over 4 h. With scaling out and parallelising, useable quantities of hundreds of micrograms for use in pharmacology studies can be synthesised simply. On-chip continuous-flow synthesis of metabolites from glucuronidation and sulfonation reactions to enable synthesis of analytical standards and study drug metabolism.
引用
收藏
页码:27696 / 27704
页数:9
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