A high-throughput, in-vitro assay for Bacillus thuringiensis insecticidal proteins

Michi Izumi Willcoxon; Jaclyn R Dennis; Sabina I Lau; Weiping Xie; You You; Song Leng; Ryan C Fong; Takashi Yamamoto

doi:10.1016/j.jbiotec.2015.10.021

A high-throughput, in-vitro assay for Bacillus thuringiensis insecticidal proteins

J Biotechnol. 2016 Jan 10:217:72-81. doi: 10.1016/j.jbiotec.2015.10.021. Epub 2015 Oct 30.

Authors

Michi Izumi Willcoxon¹, Jaclyn R Dennis², Sabina I Lau², Weiping Xie², You You², Song Leng², Ryan C Fong², Takashi Yamamoto²

Affiliations

¹ Plant Protection, Ag Biotechnology, DuPont Pioneer, 4010 Point Eden Way, Hayward, CA 94545, USA. Electronic address: michi.izumi@pioneer.com.
² Plant Protection, Ag Biotechnology, DuPont Pioneer, 4010 Point Eden Way, Hayward, CA 94545, USA.

PMID: 26524384
DOI: 10.1016/j.jbiotec.2015.10.021

Abstract

A high-throughput, in-vitro assay for Bacillus thuringiensis (Bt) insecticidal proteins designated as Cry was developed and evaluated for screening a large number of Cry protein variants produced by DNA shuffling. This automation-amenable assay exploits an insect cell line expressing a single receptor of Bt Cry proteins. The Cry toxin used to develop this assay is a variant of the Cry1Ab protein called IP1-88, which was produced previously by DNA shuffling. Cell mortality caused by the activated Bt Cry toxin was determined by chemical cell viability assay in 96/384-well microtiter plates utilizing CellTiter 96(®) obtained from Promega. A widely-accepted mode-of-action theory of certain Bt Cry proteins suggests that the activated toxin binds to one or more receptors and forms a pore through the insect gut epithelial cell apical membrane. A number of insect proteins such as cadherin-like protein (Cad), aminopeptidase-N (APN), alkaline phosphatase (ALP) and ABC transporter (ABCC) have been identified as the receptors of Bt Cry toxins. In this study, Bt Cry toxin receptors Ostrinia nubilalis (European corn borer) cadherin-like protein (On-Cad) and aminopeptidase-N 1 and 3 (On-APN1, On-APN3) and Spodoptera frugiperda (fall armyworm) cadherin-like protein (Sf-Cad) were cloned in an insect cell line, Sf21, and a mammalian cell line, Expi293F. It was observed by ligand blotting and immunofluorescence microscopy that trypsin-activated IP1-88 bound to On-Cad and On-APN1, but not Sf-Cad or On-APN3. In contrast, IP1-88 bound only to APN1 in BBMV (Brush Border Membrane Vesicles) prepared from the third and fourth-instar O. nubilalis larval midgut. The sensitivity of the recombinant cells to the toxin was then tested. IP1-88 showed no toxicity to non-recombinant Sf21 and Expi293F. Toxicity was observed only when the On-Cad gene was cloned and expressed. Sf-Cad and On-APN1 were not able to make those cells sensitive to the toxin. Since the expression of On-Cad alone was sufficient to make both insect and mammalian cells sensitive to the IP1-88 toxin, it is not likely that a secondary receptor, which may exist specifically in the Sf21 insect cell but not in the Expi293F cell, is involved in the cytotoxicity of IP1-88.

Keywords: Bacillus thuringiensis; Cadherin-like protein; Cry protein; High throughput screening; Sf21.

Publication types

Research Support, Non-U.S. Gov't

MeSH terms

Animals
Bacillus thuringiensis / chemistry*
Bacillus thuringiensis / metabolism
Bacillus thuringiensis Toxins
Bacterial Proteins / analysis*
Bacterial Toxins / analysis*
CD13 Antigens / metabolism
Cadherins / biosynthesis
Cadherins / genetics
Cell Line
Endotoxins / analysis*
Hemolysin Proteins / analysis*
High-Throughput Screening Assays / methods*
Lepidoptera
Sf9 Cells

Substances

Bacillus thuringiensis Toxins
Bacterial Proteins
Bacterial Toxins
Cadherins
Endotoxins
Hemolysin Proteins
insecticidal crystal protein, Bacillus Thuringiensis
CD13 Antigens