Production of recombinant VP1-derived virus-like particles from novel human polyomaviruses in yeast

Milda Norkiene; Jomante Stonyte; Danguole Ziogiene; Egle Mazeike; Kestutis Sasnauskas; Alma Gedvilaite

doi:10.1186/s12896-015-0187-z

Production of recombinant VP1-derived virus-like particles from novel human polyomaviruses in yeast

BMC Biotechnol. 2015 Aug 4:15:68. doi: 10.1186/s12896-015-0187-z.

Authors

Milda Norkiene¹, Jomante Stonyte², Danguole Ziogiene³, Egle Mazeike⁴, Kestutis Sasnauskas⁵, Alma Gedvilaite⁶

Affiliations

¹ Institute of Biotechnology, Vilnius University, Graiciuno 8, LT-02241, Vilnius, Lithuania. milda.norkiene@bti.vu.lt.
² Institute of Biotechnology, Vilnius University, Graiciuno 8, LT-02241, Vilnius, Lithuania. jomante@gmail.com.
³ Institute of Biotechnology, Vilnius University, Graiciuno 8, LT-02241, Vilnius, Lithuania. danguole.ziogiene@bti.vu.lt.
⁴ Institute of Biotechnology, Vilnius University, Graiciuno 8, LT-02241, Vilnius, Lithuania. egluzes@gmail.com.
⁵ Institute of Biotechnology, Vilnius University, Graiciuno 8, LT-02241, Vilnius, Lithuania. kestutis.sasnauskas@bti.vu.lt.
⁶ Institute of Biotechnology, Vilnius University, Graiciuno 8, LT-02241, Vilnius, Lithuania. agedv@ibt.lt.

Abstract

Background: Eleven new human polyomaviruses (HPyVs) have been identified in the last decade. Serological studies show that these novel HPyVs sub-clinically infect humans at an early age. The routes of infection, entry pathways, and cell tropism of new HPyVs remain unknown. VP1 proteins of polyomaviruses can assembly into virus-like particles (VLPs). As cell culturing systems for HPyV are currently not available, VP1-derived VLPs may be useful tools in basic research and biotechnological applications.

Results: Recombinant VP1-derived VLPs from 11 newly identified HPyVs were efficiently expressed in yeast. VP1 proteins derived from Merkel cell polyomavirus (MCPyV), trichodysplasia spinulosa-associated polyomavirus (TSPyV), and New Jersey polyomavirus (NJPyV) self-assembled into homogeneous similarly-sized VLPs. Karolinska Institutet polyomavirus (KIPyV), HPyV7, HPyV9, HPyV10, and St. Louis polyomavirus (STLPyV) VP1 proteins formed VLPs that varied in size with diameters ranging from 20 to 60 nm. Smaller-sized VLPs (25-35 nm in diameter) predominated in preparations from Washington University polyomavirus (WUPyV) and HPyV6. Attempts to express recombinant HPyV12 VP1-derived VLPs in yeast indicate that translation of VP1 might start at the second of two potential translation initiation sites in the VP1-encoding open reading frame (ORF). This translation resulted in a 364-amino acid-long VP1 protein, which efficiently self-assembled into typical PyV VLPs. MCPyV-, KIPyV-, TSPyV-, HPyV9-, HPyV10-, and HPyV12-derived VLPs showed hemagglutination (HA) assay activity in guinea pig erythrocytes, whereas WUPyV-, HPyV6-, HPyV7-, STLPyV- and NJPyV-derived VP1 VLPs did not.

Conclusions: The yeast expression system was successfully utilized for high-throughput production of recombinant VP1-derived VLPs from 11 newly identified HPyVs. HPyV12 VP1-derived VLPs were generated from the second of two potential translation initiation sites in the VP1-encoding ORF. Recombinant VLPs produced in yeast originated from different HPyVs demonstrated distinct HA activities and may be useful in virus diagnostics, capsid structure studies, or investigation of entry pathways and cell tropism of HPyVs until cell culture systems for new HPyVs are developed.

Publication types

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

MeSH terms

Capsid Proteins / biosynthesis*
Capsid Proteins / genetics
Capsid Proteins / immunology
Humans
Polyomavirus / genetics*
Polyomavirus / isolation & purification
Polyomavirus / pathogenicity
Polyomavirus Infections / genetics*
Polyomavirus Infections / prevention & control
Polyomavirus Infections / virology
Virion / genetics
Virion / growth & development
Virion / pathogenicity

Substances

Capsid Proteins