May 13 2021
Title:
A broadly active fucosyltransferase LmjFUT1 whose
mitochondrial localization and catalytic activity is essential in
the parasitic protozoan Leishmania
Authors: Hongjie Guo
1,
, Sebastian Damerow
2,
, Luciana Penha
1,
, Stefanie
Menzies
1,
, Gloria Polanco
1
, Hicham Zegzouti
3
, Michael A. J. Ferguson
2
,
and Stephen M. Beverley
1,
*
Affiliations:
1
Dept. of Molecular Microbiology, Washington University School
of Medicine, St. Louis, MO 63110, USA;
2
Division of Biological
Chemistry & Drug Discovery, Wellcome Trust Biocentre, College of Life
Science, University of Dundee, Dundee DD1 5EH, Scotland, United
Kingdom;
3
R&D Department, Promega Corporation, 2800 Woods
Hollow Road, Madison, WI 53711, USA.
Corresponding author: Department of Molecular Microbiology, Campus Box
8230, Washington University School of Medicine, 660 S. Euclid Ave., St.
Louis MO 63110 USA. Telephone 314-747-2630, FAX 314-747-2634,
stephen.beverley@wustl.edu
.
Author Contributions: HG, SD, SM, LP GP MAJF and SMB designed research;
HG, SD, LP, GP, and SM performed the work; HZ contributed key reagents
and methods; HG, SD, LP, GP, SM, MAJF and SMB analyzed data; and HG
MAJF and SMB wrote the paper.
Competing Interest Statement: The authors disclose no competing interests.
Classification: Biological Sciences, Microbiology
Keywords: trypanosomatid protozoan parasites, glycobiology,
glycosyltransferase, fucose, chemotherapy
This PDF file includes: Main Text including Figures 1-8 and Table 1;
Supplemental Figures 1-6 and Supplemental Tables 1-2
was not certified by peer review) is the author/funder. All rights reserved. No reuse allowed without permission.
The copyright holder for this preprint (whichthis version posted May 13, 2021. ; https://doi.org/10.1101/2021.05.10.443387doi: bioRxiv preprint
ABSTRACT (246 words)
Glycoconjugates play major roles in the infectious cycle of the trypanosomatid parasite
Leishmania. While GDP-Fucose synthesis is essential (Guo et al 2017), fucosylated
glycoconjugates have not been reported in Leishmania major. Four predicted fucosyltransferases
appear conventionally targeted to the secretory pathway; SCA1/2 play a role in side-chain
modifications of lipophosphoglycan, while gene deletion studies here showed that FUT2 and
SCAL were not essential. Unlike most eukaryotic glycosyltransferases, the predicted α 1-2
fucosyltransferase encoded by FUT1 localized to the mitochondrion. A quantitative ‘plasmid
segregation’ assay, expressing FUT1 from the multicopy episomal pXNG vector in a
chromosomal null ∆fut1
-
background, established that FUT1 is essential. Similarly “plasmid
shuffling” confirmed that both enzymatic activity and mitochondrial localization were required
for viability, comparing import-blocked or catalytically inactive enzymes respectively.
Enzymatic assays of tagged proteins expressed in vivo or of purified recombinant FUT1 showed
it had a broad fucosyltransferase activity including glycan and peptide substrates. Unexpectedly
a single rare ∆fut1
-
s
segregant (∆fut1
s
) was obtained in rich media, which showed severe growth
defects accompanied by mitochondrial dysfunction and loss, all of which were restored upon
FUT1 re-expression. Thus, FUT1 along with the similar Trypanosoma brucei enzyme TbFUT1
(Bandini et al 2021) joins the eukaryotic O-GlcNAc transferase isoform as one of the few
glycosyltransferases acting within the mitochondrion. Trypanosomatid mitochondrial FUT1s
may offer a facile system for probing mitochondrial glycosylation in a simple setting and their
essentiality renders it an attractive target for chemotherapy of these serious human pathogens.
was not certified by peer review) is the author/funder. All rights reserved. No reuse allowed without permission.
The copyright holder for this preprint (whichthis version posted May 13, 2021. ; https://doi.org/10.1101/2021.05.10.443387doi: bioRxiv preprint
Significance Statement (120 words)
Abundant surface glycoconjugates play key roles in the infectious cycle of protozoan parasites
including Leishmania. Through defining biosynthetic pathways we identified a
fucosyltransferase FUT1 that was localized to the parasite mitochondrion, an atypical
compartment for glycosyltransferases. FUT1 was essential for normal growth, requiring both
mitochondrial localization and enzymatic activity. Loss of FUT1 in a unique segregant showed
extensive mitochondrial defects. Enzymatic tests showed FUT1 could fucosylate glycan and
peptide substrates in vitro, although as yet the native substrate is unknown. Trypanosomatid
mitochondrial FUT1s may offer a facile system in the future for probing mitochondrial
glycosylation in a setting uncomplicated by multiple isoforms targeted to diverse compartments,
and its essentiality renders it an attractive target for chemotherapy of these deadly parasites.
was not certified by peer review) is the author/funder. All rights reserved. No reuse allowed without permission.
The copyright holder for this preprint (whichthis version posted May 13, 2021. ; https://doi.org/10.1101/2021.05.10.443387doi: bioRxiv preprint
Introduction
Leishmania is a widespread human pathogen, with more than 1.7 billion people at risk,
several hundred million infected, and with 12 million showing active disease ranging from mild
cutaneous lesions to severe disfiguring or ultimate lethal outcomes (2-4). The Leishmania
infectious cycle alternates between extracellular promastigote in the midgut of sand flies and
intracellular amastigote residing within macrophages of the mammalian host, where it survives
and proliferates in highly hostile environments. These parasites have evolved specific
mechanisms enabling them to endure these adverse conditions, including a dense cell surface
glycocalyx composed of lipophosphoglycan (LPG), glycosylphosphatidylinositol (GPI) anchored
proteins (GP63 and GP46), glycosylinositolphospholipids (GIPLs) and secreted glycoconjugates
such as proteophosphoglycan (PPG) and secreted acid phosphatase (sAP) (reviewed in 5; 6-8).
One prominent feature of LPG, PPGs and sAPs is the presence of disaccharide phosphate
repeating units ([6Gal(β)1,4)Man(α1)-PO
4
]), also termed phosphoglycan or PG repeats.
Our lab has focused on both forward and reverse genetic approaches to map out
glycoconjugate synthesis in Leishmania, emphasizing genes impacting the glycocalyx (9, 10) as
well as ether lipids and sphingolipids (11, 12). These studies have provided powerful tools
leading to new insights on the requirements for LPG and related phosphoglycan -bearing
molecules in both parasite stages within the mammalian and sand fly hosts (6, 7, 13-19).
In several Leishmania species modifications of the dominant PG repeats of LPG and PPG
play key roles in the insect stages in mediating both the attachment and release of promastigotes
and metacyclics, respectively, from the sand fly midgut via binding to midgut receptors there
(20). In L. major strain FV1 (LmjF), β1-3 galactosyl modifications of the PG repeating units
enable replicating promastigotes to bind to the midgut lectin PpGalec, while addition of D-
Arabinopyranose (D-Arap) to the side-chain galactosyl residues block this interaction and allow
was not certified by peer review) is the author/funder. All rights reserved. No reuse allowed without permission.
The copyright holder for this preprint (whichthis version posted May 13, 2021. ; https://doi.org/10.1101/2021.05.10.443387doi: bioRxiv preprint
release of parasites for subsequent transmission (20-22). Accordingly, we used forward genetic
analysis to identify a large family of LPG side chain galactosyltransferases (SCG1-7) and D-
Arabinopyranosyltransferases (SCA1/2) mediating these key modifications (22-27).
As D-Arap is relatively uncommon in nature (28), we were motivated to explore its
synthetic pathway. Previously we identified two genes showing strong homology to the
bifunctional Bacteroides protein FKP mediating synthesis of GDP-L-Fucose (GDP-Fuc) through
successive kinase and pyrophosphorylase steps (29, 30). Many enzymes using L-Fucose will
also accept D-Arap (which differ only by the 6-methyl group), and assays of the two
recombinant Leishmania proteins showed that indeed one could synthesize both GDP-D-Arap
and GDP-Fuc (AFKP; LmjF.16.0480), while the second could only synthesize GDP- Fuc (FKP;
LmjF.16.0440; (30)). These data were consistent with studies showing the presence of both
GDP-Fuc and GDP-Arap in Leishmania (31). Correspondingly, genetic studies showed that
knockouts of AFKP completely abrogated GDP-Arap and arabinosylated LPG synthesis, while
knockouts of FKP showed little effect (30). However, we were unable to knockout both genes
simultaneously, suggesting an unanticipated role for GDP-Fuc. That the essential role of
A/FKPs depended on GDP-Fucose was established when GDP-Fuc but not GDP-Arap was
provided through expression of the two de novo GDP-Fucose enzymes from Trypanosoma
brucei, GDP-mannose 4,6-dehydratase (GMD) and GDP-Fuc synthetase, also known as GDP-4-
dehydro-6-deoxy-D-mannose epimerase/reductase (GMER) (32). Similarly the loss of de novo
GDP-fucose synthesis was also lethal in T. brucei, which lacks the FKP salvage pathway (32).
The essentiality of GDP-Fuc was unexpected since there are few reports of fucosylated
molecules in Leishmania. One is a “Fucose Mannose Ligand” from L. donovani (33) for which a
definitive structure is lacking. Several proteins were predicted to be fucosylated from mass
was not certified by peer review) is the author/funder. All rights reserved. No reuse allowed without permission.
The copyright holder for this preprint (whichthis version posted May 13, 2021. ; https://doi.org/10.1101/2021.05.10.443387doi: bioRxiv preprint