Engineering the Escherichia coli Nitroreductase NfsA to Create a Flexible Enzyme-Prodrug Activation System

Abigail V Sharrock; Sarah P McManaway; Michelle H Rich; Jeff S Mumm; Ian F Hermans; Moana Tercel; Frederik B Pruijn; David F Ackerley

doi:10.3389/fphar.2021.701456

Engineering the Escherichia coli Nitroreductase NfsA to Create a Flexible Enzyme-Prodrug Activation System

Front Pharmacol. 2021 Jun 7:12:701456. doi: 10.3389/fphar.2021.701456. eCollection 2021.

Authors

Abigail V Sharrock^{1

2

3}, Sarah P McManaway⁴, Michelle H Rich¹, Jeff S Mumm⁵, Ian F Hermans^{1

3

6}, Moana Tercel^{3

4}, Frederik B Pruijn^{3

4}, David F Ackerley^{1

2

3}

Affiliations

¹ School of Biological Sciences, Victoria University of Wellington, Wellington, New Zealand.
² Centre for Biodiscovery, Victoria University of Wellington, Wellington, New Zealand.
³ Maurice Wilkins Centre for Molecular Biodiscovery, Auckland, New Zealand.
⁴ Auckland Cancer Society Research Centre, The University of Auckland, Auckland, New Zealand.
⁵ The Wilmer Eye Institute, Johns Hopkins University, Baltimore, MD, United States.
⁶ Malaghan Institute of Medical Research, Wellington, New Zealand.

Abstract

Bacterial nitroreductase enzymes that can efficiently convert nitroaromatic prodrugs to a cytotoxic form have numerous applications in targeted cellular ablation. For example, the generation of cytotoxic metabolites that have low bystander potential (i.e., are largely confined to the activating cell) has been exploited for precise ablation of specific cell types in animal and cell-culture models; while enzyme-prodrug combinations that generate high levels of bystander cell killing are useful for anti-cancer strategies such as gene-directed enzyme-prodrug therapy (GDEPT). Despite receiving substantial attention for such applications, the canonical nitroreductase NfsB from Escherichia coli has flaws that limit its utility, in particular a low efficiency of conversion of most prodrugs. Here, we sought to engineer a superior broad-range nitroreductase, E. coli NfsA, for improved activity with three therapeutically-relevant prodrugs: the duocarmycin analogue nitro-CBI-DEI, the dinitrobenzamide aziridine CB1954 and the 5-nitroimidazole metronidazole. The former two prodrugs have applications in GDEPT, while the latter has been employed for targeted ablation experiments and as a precise 'off-switch' in GDEPT models to eliminate nitroreductase-expressing cells. Our lead engineered NfsA (variant 11_78, with the residue substitutions S41Y, L103M, K222E and R225A) generated reduced metabolites of CB1954 and nitro-CBI-DEI that exhibited high bystander efficiencies in both bacterial and 2D HEK-293 cell culture models, while no cell-to-cell transfer was evident for the reduced metronidazole metabolite. We showed that the high bystander efficiency for CB1954 could be attributed to near-exclusive generation of the 2-hydroxylamine reduction product, which has been shown in 3D cell culture to cause significantly greater bystander killing than the 4-hydroxylamine species that is also produced by NfsB. We similarly observed a high bystander effect for nitro-CBI-DEI in HCT-116 tumor spheroids in which only a small proportion of cells were expressing variant 11_78. Collectively, our data identify variant 11_78 as a broadly improved prodrug-activating nitroreductase that offers advantages for both targeted cellular ablation and suicide gene therapy applications.

Keywords: BDEPT; GDEPT; bystander effect; enzyme-prodrug therapy; nitroreductase (NTR); targeted cell ablation.

Grants and funding

R01 OD020376/OD/NIH HHS/United States