A new method for in vitro feeding of Rhipicephalus australis (formerly Rhipicephalus microplus) larvae: a valuable tool for tick vaccine development

Jos J A Trentelman; Jos A G M Kleuskens; Jos van de Crommert; Theo P M Schetters

doi:10.1186/s13071-017-2081-0

A new method for in vitro feeding of Rhipicephalus australis (formerly Rhipicephalus microplus) larvae: a valuable tool for tick vaccine development

Parasit Vectors. 2017 Mar 23;10(1):153. doi: 10.1186/s13071-017-2081-0.

Authors

Jos J A Trentelman¹, Jos A G M Kleuskens², Jos van de Crommert³, Theo P M Schetters^{4

5}

Affiliations

¹ Center for Experimental and Molecular Medicine, Academic Medical Center Amsterdam, meibergdreef 9, 1105, AZ, Amsterdam, Netherlands. j.j.trentelman@amc.uva.nl.
² Center for Experimental and Molecular Medicine, Academic Medical Center Amsterdam, meibergdreef 9, 1105, AZ, Amsterdam, Netherlands.
³ Aduro Biotech Europe, Kloosterstraat 9, 1101, RX, Boxmeer, Netherlands.
⁴ ProtActivity R&D, Sering 36, 5432, DD, Cuijk, Netherlands.
⁵ ClinVet International, Uitzich Road, Bainsvlei, 9338, Bloemfontein, South Africa.

Abstract

Background: Rhipicephalus microplus is a hard tick that has a major impact on cattle health in tropical and subtropical regions because it feeds on cattle and is implicated in the transmission of pathogens that cause diseases such as bovine anaplasmosis and babesiosis. Presently, acaricides are used to control tick infestation but this is becoming increasingly less effective due to the emergence of tick strains that are resistant to one or more classes of acaricides. Anti-tick vaccines are a promising alternative to control tick infestation in cattle. The life-cycle and host preference of R. microplus, however, makes vaccine research in cattle costly and would therefore greatly benefit from an in vitro screening system.

Methods: To this aim, a stacked 24-well in vitro feeding system was designed in which the blood meal was administered in a chamber on top of the compartment containing the ticks, exploiting their anti-gravitational tendency. Both compartments were separated by a special feeding membrane, which was made by applying a silicone mixture to a gold beater's skin (baudruche membrane) with a paint roller to create a slightly uneven surface of 17-40 μm variable thickness. To further stimulate feeding, the membrane was treated with bovine hair extract and the unit was placed at 37 °C with 90% RH and 5% CO₂.

Results: Using this set-up with Rhipicephalus australis (formerly Rhipicephalus microplus), a larval engorgement rate of up to 71% could be achieved. The larvae could successfully feed on blood, but also on serum. The latter allows easy screening of the effect of sera that are raised against tick proteins on feeding. As an example, serum from cattle that were vaccinated with the Bm86 midgut protein of R. microplus significantly reduced larval engorgement rates by 42%.

Conclusion: The in vitro feeding system's high throughput design and its ability to measure statistically significant anti-tick effects in sera from immunized cattle enables screening of multiple vaccine candidates in a cost-effective manner.

Keywords: Artificial tick feeding; In vitro screening; Larvae; Rhipicephalus australis; Rhipicephalus microplus.

MeSH terms

Animal Feed
Animals
Entomology / methods*
Feeding Methods*
Larva / growth & development
Rhipicephalus / growth & development*
Temperature