High‐Throughput Method for Determining the Enantioselectivity of Enzyme‐Catalyzed Hydroxylations Based on Mass Spectrometry

Chen, Yongzheng; Tang, Weng Lin; Mou, Jie; Li, Zhi

doi:10.1002/anie.201001772

Cited by 46 publications

(15 citation statements)

References 95 publications

(11 reference statements)

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“…Li and coworkers reported a method to determine the enantioselectivity of C–H/D hydroxylation reactions conducted on deuterium-substituted substrates using mass spectrometry (GC/MS or LC/MS). 49 We envisioned that deuterated tryptamines could be used in a similar fashion to identify RebH variants with altered regioselectivity. RebH halogenates tryptamine with the same high 7-selectivity that it exhibits on tryptophan, 33 but deuterated tryptamines are more readily prepared than the corresponding tryptophans.…”

Section: Resultsmentioning

confidence: 99%

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Directed evolution of RebH for catalyst-controlled halogenation of indole C–H bonds

et al. 2016

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RebH variants capable of chlorinating substituted indoles ortho-, meta-, and para- to the indole nitrogen were evolved by directly screening for altered selectivity on deuterium-substituted probe substrates using mass spectrometry. This systematic approach allowed for rapid accumulation of beneficial mutations using simple adaptive walks and should prove generally useful for altering and optimizing the selectivity of C-H functionalization catalysts. Analysis of the beneficial mutations showed that structure-guided selection of active site residues for targeted mutagenesis can be complicated either by activity/selectivity tradeoffs that reduce the possibility of detecting such mutations or by epistatic effects that actually eliminate the benefits of a mutation in certain contexts. As a corollary to this finding, the precise manner in which the beneficial mutations identified led to the observed changes in RebH selectivity is not clear. Docking simulations suggest that tryptamine binds to these variants as tryptophan does to native halogenases, but structural studies will be required to confirm these models and shed light on how particular mutations impact tryptamine binding. Similar directed evolution efforts on other enzymes or artificial metalloenzymes could enable a wide range of C-H functionalization reactions.

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Section: Resultsmentioning

confidence: 99%

“…S1 and S2 † ), so rate differences of the isotopomers did not have to be taken into account. 49 Halogenation selectivity could be reliably determined by MALDI-MS analysis of crude reaction mixtures arrayed onto a standard 384-spot sample targets, which allowed for rapid evaluation of halogenase libraries.…”

Section: Resultsmentioning

confidence: 99%

Directed evolution of RebH for catalyst-controlled halogenation of indole C–H bonds

et al. 2016

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“…Optically active benzylic bromides have been reported to be prone to racemisation 1c,e,10. For instance, a sample of ( R )-1-(bromoethyl)benzene having 88% ee kept at 0 °C was shown to fully racemise within 8 hours 1 c .…”

Section: Resultsmentioning

confidence: 99%

“…The above methods showcase the recent progress made in the deoxybromination of alkyl alcohols; however, challenges remain such as alkene side product formation from elimination sensitive bromides, limited scope and functional group tolerance, difficulties in removing by-products such as phosphine oxides, requirement of multiple reagents and bromide racemisation from optically active alkyl alcohols 6a,10…”

Section: Introductionmentioning

confidence: 99%

Sulphide as a leaving group: highly stereoselective bromination of alkyl phenyl sulphides

et al. 2019

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“…In short, we have introduced the PECANm ass-spectrometric enzyme activity assay,and demonstrated its suitability for high-throughput screening of P450s in complex matrices, such as cell lysates and microsomes.W hile we have demonstrated the applicability of PECANonly to P450s,webelieve that, after the appropriate method development, this technology could be applicable to any enzyme (or set of enzymatic reactions), that changes the mass of its substrate.F urthermore,i tm ay be possible to monitor isomerization reactions through the application of tandem MS,o re nantioselective reactions through the use of isotopically labeled substrates. [47] As expected from any high-throughput assay,o ur PECAN screen yielded some false positives,a nd we re-screened as mall subset of the library using low-throughput analytical technologies to verify the hits,asisroutine in this field. Like spectrometric assays,t he PECANt echnology requires the synthesis of as pecialized probe and enzymatic reactions are performed in microtiter plates.Therefore,weexpect PECAN to have roughly equivalent throughput to-and act as ac omplementary method to-spectrometric assays.W e expect PECANt ob eavaluable technology for drug discovery or directed-evolution campaigns that focus on enzymes for which no high-throughput screen currently exists.…”

Section: Angewandte Chemiementioning

confidence: 99%

A High‐Throughput Mass Spectrometric Enzyme Activity Assay Enabling the Discovery of Cytochrome P450 Biocatalysts

et al. 2019

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Assaying for enzymatic activity is ap ersistent bottlenecki nb iocatalyst and drug development. Existing high-throughput assays for enzyme activity tend to be applicable only to an arrowr ange of biochemical transformations, whereas universal enzyme characterization methods usually require chromatography to determine substrate turnover, greatly diminishing throughput. We present an enzyme activity assayt hat allows the high-throughput mass-spectrometric detection of enzyme activity in complex matrices without the need for ac hromatographic step.T his technology,w hichw e call probing enzymes with click-assisted NIMS (PECAN), can detect the activity of medically and biocatalytically significant cytochrome P450s in cell lysate,m icrosomes,a nd bacteria. Using this approach, acytochrome P450 BM3 mutant library was successfully screened for the ability to catalyze the oxidation of the sesquiterpene valencene.

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High‐Throughput Method for Determining the Enantioselectivity of Enzyme‐Catalyzed Hydroxylations Based on Mass Spectrometry

Abstract: Up to speed: An accurate, sensitive, high‐throughput, and simple method for measuring the product ee value of enzyme‐catalyzed hydroxylations (see scheme) is based on the use of enantiopure or enantioenriched deuterated substrates and mass spectrometric detection.

Cited by 46 publications

References 95 publications

Directed evolution of RebH for catalyst-controlled halogenation of indole C–H bonds

Directed evolution of RebH for catalyst-controlled halogenation of indole C–H bonds

Sulphide as a leaving group: highly stereoselective bromination of alkyl phenyl sulphides

A High‐Throughput Mass Spectrometric Enzyme Activity Assay Enabling the Discovery of Cytochrome P450 Biocatalysts

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