Virulence factor RNA transcript expression in the Leishmania Viannia subgenus: influence of species, isolate source, and Leishmania RNA virus-1

Ruwandi Kariyawasam; Avinash N Mukkala; Rachel Lau; Braulio M Valencia; Alejandro Llanos-Cuentas; Andrea K Boggild

doi:10.1186/s41182-019-0153-x

Virulence factor RNA transcript expression in the Leishmania Viannia subgenus: influence of species, isolate source, and Leishmania RNA virus-1

Trop Med Health. 2019 Apr 11:47:25. doi: 10.1186/s41182-019-0153-x. eCollection 2019.

Authors

Ruwandi Kariyawasam¹, Avinash N Mukkala¹, Rachel Lau², Braulio M Valencia^{3

4}, Alejandro Llanos-Cuentas^{3

5}, Andrea K Boggild^{1

2

6

7}

Affiliations

¹ 1Institute of Medical Sciences, University of Toronto, Toronto, ON Canada.
² 2Public Health Ontario Laboratory, Toronto, ON Canada.
³ Instituto de Medicina Tropical "Alejandro von Humboldt", Lima, Peru.
⁴ 7Viral Immunology Systems Program, Kirby Institute, University of New South Wales, Sydney, Australia.
⁵ 4Facultad de Salud Pública y Administración, Universidad Peruana Cayetano Heredia, Lima, Peru.
⁶ 5Department of Medicine, University of Toronto, Toronto, ON Canada.
⁷ 6Tropical Disease Unit, Toronto General Hospital, 200 Elizabeth Street, 13EN-218, Toronto, ON M5G 2C4 Canada.

Abstract

Background: Leishmania RNA virus-1 (LRV1) is a double-stranded RNA virus identified in 20-25% of Viannia-species endemic to Latin America, and is believed to accelerate cutaneous to mucosal leishmaniasis over time. Our objective was to quantify known virulence factor (VF) RNA transcript expression according to LRV1 status, causative species, and isolate source.

Methods: Eight cultured isolates of Leishmania were used, four of which were LRV1-positive (Leishmania Viannia braziliensis [n = 1], L. (V.) guyanensis [n = 1], L. (V.) panamensis [n = 2]), and four were LRV1-negative (L. (V.) panamensis [n = 3], L. (V.) braziliensis [n = 1]). Promastigotes were inoculated into macrophage cultures, and harvested at 24 and 48 h. RNA transcript expression of hsp23, hsp70, hsp90, hsp100, mpi, cpb, and gp63 were quantified by qPCR.

Results: RNA transcript expression of hsp100 (p = 0.012), cpb (p = 0.016), and mpi (p = 0.022) showed significant increases from baseline pure culture expression to 24- and 48-h post-macrophage infection, whereas hsp70 (p = 0.004) was significantly decreased. A trend toward increased transcript expression of hsp100 at baseline in isolates of L. (V.) panamensis was noted. Pooled VF RNA transcript expression by L. (V.) panamensis isolates was lower than that of L. (V.) braziliensis and L. (V.) guyananesis at 24 h (p = 0.03). VF RNA transcript expression did not differ by LRV1 status, or source of cultured isolate at baseline, 24, or 48 h; however, a trend toward increased VF RNA transcript expression of 2.71- and 1.93-fold change of mpi (p = 0.11) and hsp90 (p = 0.11), respectively, in LRV1 negative isolates was noted. Similarly, a trend toward lower levels of overall VF RNA transcript expression in clinical isolates (1.15-fold change) compared to ATCC® strains at 24 h was noted (p = 0.07).

Conclusions: Our findings suggest that known VF RNA transcript expression may be affected by the process of macrophage infection. We were unable to demonstrate definitively that LRV-1 presence affected VF RNA transcript expression in the species and isolates studied. L. (V.) guyanensis and L. (V.) braziliensis demonstrated higher pooled VF RNA transcript expression than L. (V.) panamensis; however, further analyses of protein expression to corroborate this finding are warranted.

Keywords: American tegumentary leishmaniasis; Leishmania RNA Virus-1 (LRV1); Leishmania Viannia braziliensis; Virulence factor.