PLoS Pathogens (Mar 2023)

The Trypanosoma brucei MISP family of invariant proteins is co-expressed with BARP as triple helical bundle structures on the surface of salivary gland forms, but is dispensable for parasite development within the tsetse vector.

  • Aitor Casas-Sanchez,
  • Raghavendran Ramaswamy,
  • Samïrah Perally,
  • Lee R Haines,
  • Clair Rose,
  • Marcela Aguilera-Flores,
  • Susana Portillo,
  • Margot Verbeelen,
  • Shahid Hussain,
  • Laura Smithson,
  • Cristina Yunta,
  • Michael J Lehane,
  • Sue Vaughan,
  • Jan van den Abbeele,
  • Igor C Almeida,
  • Martin J Boulanger,
  • Álvaro Acosta-Serrano

DOI
https://doi.org/10.1371/journal.ppat.1011269
Journal volume & issue
Vol. 19, no. 3
p. e1011269

Abstract

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Trypanosoma brucei spp. develop into mammalian-infectious metacyclic trypomastigotes inside tsetse salivary glands. Besides acquiring a variant surface glycoprotein (VSG) coat, little is known about the metacyclic expression of invariant surface antigens. Proteomic analyses of saliva from T. brucei-infected tsetse flies identified, in addition to VSG and Brucei Alanine-Rich Protein (BARP) peptides, a family of glycosylphosphatidylinositol (GPI)-anchored surface proteins herein named as Metacyclic Invariant Surface Proteins (MISP) because of its predominant expression on the surface of metacyclic trypomastigotes. The MISP family is encoded by five paralog genes with >80% protein identity, which are exclusively expressed by salivary gland stages of the parasite and peak in metacyclic stage, as shown by confocal microscopy and immuno-high resolution scanning electron microscopy. Crystallographic analysis of a MISP isoform (MISP360) and a high confidence model of BARP revealed a triple helical bundle architecture commonly found in other trypanosome surface proteins. Molecular modelling combined with live fluorescent microscopy suggests that MISP N-termini are potentially extended above the metacyclic VSG coat, and thus could be tested as a transmission-blocking vaccine target. However, vaccination with recombinant MISP360 isoform did not protect mice against a T. brucei infectious tsetse bite. Lastly, both CRISPR-Cas9-driven knock out and RNAi knock down of all MISP paralogues suggest they are not essential for parasite development in the tsetse vector. We suggest MISP may be relevant during trypanosome transmission or establishment in the vertebrate's skin.