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Toxoplasma TgATG9 is critical for autophagy and long-term persistence in tissue cysts - PubMed

️Fri Jan 01 2021

doi: 10.7554/eLife.59384.

Geetha Kannan¹, Isabelle Coppens², Fengrong Wang¹, Hoa Mai Nguyen³, Aude Cerutti³, Einar B Olafsson¹, Patrick A Rimple¹, Tracey L Schultz¹, Nayanna M Mercado Soto¹, Manlio Di Cristina^{1

4}, Sébastien Besteiro³, Vern B Carruthers¹

Affiliations

PMID: 33904393
PMCID: PMC8128441
DOI: 10.7554/eLife.59384

Toxoplasma TgATG9 is critical for autophagy and long-term persistence in tissue cysts

David Smith et al. Elife. 2021.

Abstract

Many of the world's warm-blooded species are chronically infected with Toxoplasma gondii tissue cysts, including an estimated one-third of the global human population. The cellular processes that permit long-term persistence within the cyst are largely unknown for T. gondii and related coccidian parasites that impact human and animal health. Herein, we show that genetic ablation of TgATG9 substantially reduces canonical autophagy and compromises bradyzoite viability. Transmission electron microscopy revealed numerous structural abnormalities occurring in ∆atg9 bradyzoites. Intriguingly, abnormal mitochondrial networks were observed in TgATG9-deficient bradyzoites, some of which contained numerous different cytoplasmic components and organelles. ∆atg9 bradyzoite fitness was drastically compromised in vitro and in mice, with very few brain cysts identified in mice 5 weeks post-infection. Taken together, our data suggests that TgATG9, and by extension autophagy, is critical for cellular homeostasis in bradyzoites and is necessary for long-term persistence within the cyst of this coccidian parasite.

Keywords: ATG9; Toxoplasma gondii; apicomplexa; chronic infection; infectious disease; microbiology; parasite; protozoan.

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Conflict of interest statement

DS, GK, IC, FW, HN, AC, EO, PR, TS, NM, MD, SB, VC No competing interests declared

Figures

**Figure 1.. Phylogenetic conservation and adaptation of autophagy-related proteins in alveolates.**
(A) Reciprocal BLAST hits to *Toxoplasma gondii* autophagy-related proteins detected in different alveolates. The inverse logarithm of the E value (−logE) from each hit with a corresponding *T. gondii* protein is plotted in a heat map to indicate the extent to which *T. gondii* autophagy-related proteins are conserved among other alveolates. A higher −logE value indicates a closer match to *T. gondii* orthologs. The number of orthologs is shown in the corresponding cell if more than one ortholog was identified. Boxes with a cross indicate no matching ortholog was identified. (B) Working models of canonical autophagy and apicoplast segregation mediated by a subset of autophagy-related proteins. Autophagy-related proteins are color-coded according to phenotype scores indicated in the scale. Autophagy proteins adapted for apicoplast maintenance tend to have negative phenotype scores in tachyzoites, based on a genome-wide CRISPR/Cas9 screen in *T. gondii* (Sidik et al., 2016), indicating they are essential for parasite survival in the acute stage of infection. Autophagy-related proteins that have a role in canonical autophagy and have not been adapted for apicoplast maintenance tend to have neutral or positive phenotype scores, indicating canonical autophagy is a non-essential cellular pathway in acute stage parasites.

**Figure 2.. TgATG8 is required for efficient autophagosome production in *Toxoplasma gondii* bradyzoites.**
(A) Stage-specific expression and fluorescent tagging of TgATG8 was achieved by insertion of the tachyzoite-specific *TgSAG1* promoter and a GFP-coding sequence immediately upstream of the *TgATG8* gene. Site-specific insertion of the DHFR-pSAG1-mGFP repair template was performed by homology-directed repair. (B) Polymerase chain reaction (PCR) analysis confirmed the repair template had been inserted at the correct locus to generate a *T. gondii* strain in which *TgATG8* expression was driven by the *TgSAG1* promoter (*S/ATG8*). Stage-specific expression of GFP-TgATG8 in tachyzoites (Tz) but not bradyzoites (Bz) was confirmed by immunofluorescence microscopy (C) and western blotting (D). GFP-TgATG8 signal overlapped with the apicoplast marker TgCPN60 (a native luminal apicoplast chaperone), indicating correct localization to the apicoplast. Dashed lines outline individual parasites in the tachyzoite images and the limits of cysts on the bradyzoite images. (E) Fluorescent staining of in vitro differentiated cysts with the bradyzoite specific marker TgBAG1 and the autolysosome detection reagent CytoID. Phase contrast images indicate the development of dark puncta in LHVS-treated bradyzoites. Scale bar, 10 µm. (F) Viability of Pru∆*hxg* and S/ATG8 bradyzoites isolated after 28 days of differentiation, as indicated by their application to fresh monolayers for plaque formation.

**Figure 3.. TgATG9 is required for efficient autophagosome production in *T. gondii* bradyzoites.**
(A) Phase contrast images showing that the development of dark puncta in in vitro differentiated bradyzoites following LHVS treatment is dependent on the expression of TgATG9. Arrowheads indicate a subset of dark puncta. Scale bar, 10 µm. (B) Quantification of dark puncta size. Each dot represents the mean size of puncta within one cyst. Data are merged from six biological replicates, with a minimum of 22 cysts analyzed per sample type, per biological replicate, and a minimum total of 242 cysts analyzed per sample type across all biological replicates. (C) CytoID staining of autolysosomes in in vitro differentiated bradyzoite cysts. Arrowheads indicate an arbitrary subset of dark puncta and the corresponding CytoID-positive structures. Scale bar, 5 µm. Quantification of the size (D) and number (E) of CytoID-positive structures in in vitro differentiated bradyzoites. Each dot represents the average puncta measurement within a single cyst. Data are merged from three biological replicates, with a minimum total of 81 cysts analyzed per sample type across three biological replicates. Cysts were identified by Dolichos lectin staining and measurements of dark puncta and CytoID were made exclusively within Dolichos lectin-positive regions. For panels B, D, and E, bars represent mean ± SD. Statistical comparisons were done using a Kruskal-Wallis test with Dunn’s multiple comparisons. Statistical significance is indicated as follows: **p<0.01; ***p<0.001; ****p<0.0001. Non-significant differences are not indicated. Statistical analysis is only shown for comparisons that have one variable, that is, different strain or different treatment.

**Figure 3—figure supplement 1.. Targeted deletion and genetic complementation of TgATG9.**
(A) The *TgATG9* gene was replaced with an HXGPRT selectable marker by homology-directed repair facilitated by CRISPR-Cas9 double-strand break directed via a single sgRNA (guide). Primers used to validate correct integration are indicated as red arrows. (B) Polymerase chain reaction (PCR) validation of ∆*atg9* parasites using the primers indicated in panel A. (C) Real-time quantitative PCR (qRT-PCR) analysis showing relative transcript levels of *TgATG9* in Pru∆*hxg*, ∆*atg9*, and ∆*atg9ATG9* strains. (D) Western blots of tachyzoites (Tz) and bradyzoites (Bz) showing re-expression of TgATG9-HA in both stages of ∆*atg9ATG9* parasites detected with anti-HA antibodies. The same blot was stripped and reprobed with anti-TgMIC2 as a loading control. (E) Immunofluorescence assay (IFA) showing re-expression of TgATG9-HA in a newly invaded tachyzoite. Scale bar, 100 nm.

**Figure 4.. Canonical autophagy is required for normal bradyzoite morphology and cell division.**
(A) Quantification of cyst size based on staining for the cyst wall with Dolichos lectin. Each dot represents the size of one cyst. Data are merged from three biological replicates, each with a minimum of 52 cysts analyzed per sample type, per biological replicate, and a minimum total of 199 cysts analyzed per sample type across three biological replicates. Bars indicate mean ± SD. Statistical comparisons were done using a Kruskal-Wallis test with Dunn’s multiple comparisons. Significance is indicated as **p<0.01; ****p<0.0001. Non-significant differences are not indicated. (B) Immunofluorescence imaging of bradyzoites stained with anti-TgIMC1 revealed disorganization of the inner membrane complex in ∆*atg9* parasites and a ‘bloating’ phenotype. Scale bar, 10 µm. (C) Transmission electron microscopy (TEM) showing a cyst containing normally developed bradyzoites from Pru∆*hxg* (a) and aberrant ∆*atg9* bradyzoites (b), with highly vacuolized, dying parasites (asterisks) or abnormally enlarged nuclear envelope (arrow). P, parasite. (D) TEM showing normal endodyogeny for Pru∆*hxg* bradyzoites with a nascent daughter containing well-organized organelles surrounded by the IMC (yellow arrowhead in panel a), and aberrant parasite division with poor packaging of organelles by the IMC (b), resulting in enlarged multinucleated ∆*atg9* bradyzoites (pseudocolorized parasite, c). Note that Pru∆*hxg* and mutant parasites are shown at the same magnification for direct comparison. All scales bars are 1 μm.

**Figure 5.. A lack of canonical autophagy leads to ultrastructural abnormalities in the vacuolar compartment (VAC) of bradyzoites.**
(A) Transmission electron microscopy (TEM) showing a normal VAC (V) in Pru∆*hxg* bradyzoites (panel a). Three types of VAC abnormalities were observed in ∆*atg9* bradyzoites: a very enlarged electron-lucent (e-lucent) compartment (panel b), small electron-dense vesicles (panel c), or a very enlarged electron-dense compartment (panel d). (B) TEM of VAC in Pru∆*hxg* and ∆*atg9* bradyzoites treated with LHVS showing for both strains very large VAC with e-lucent content (panels a and c) or electron-dense content (panels b and d). All scales bars are 1 μm.

**Figure 6.. Autophagic structures and abnormal mitochondria in Δ*atg9* bradyzoites.**
(A) Transmission electron microscopy (TEM) of ∆*atg9* parasites showing a double-membrane structure containing cytoplasmic components including endoplasmic reticulum (ER). (B) TEM showing a normal mitochondrion in Pru∆*hxg* bradyzoites. (C) TEM of ∆*atg9* bradyzoites presenting thin mitochondria (m) in a horseshoe conformation with bulbous ends, wherein cristae can be seen. Nucleus (n) is denoted. (D) TEM of ∆*atg9* parasites revealing mitochondrial profiles (m) enveloping many organelles, including ER, dense granules (DG), micronemes (mi), mitochondria (m), and lipid droplets (LD). (E) Examples of ER and mitochondrial section wrapped by the mitochondrion after bradyzoite treatment with LHVS. Inset of the lower panel illustrates the four membranes observed in such structures. All TEM scale bars are 500 nm. Mitochondria morphology scores (relative F₁F₀ATPase score) for Pru∆*hxg*, ∆*atg9*, and ∆*atg9ATG9* parasites 1 and 3 (F) or 6 and 8 (G) days after the addition of alkaline media to stimulate differentiation from the tachyzoite to bradyzoite life stage. Relative F₁F₀ ATPase Score was normalized to the Pru∆*hxg* strain within each time point. Each data point represents one cyst. Solid lines represent the mean from three biological replicates. Statistical significance between samples was determined using a Kruskal-Wallis test with Dunn’s multiple comparisons and is indicated with **p<0.01 or ***p<0.001. (H) Immunofluorescence imaging of bradyzoites stained with α-F₁F₀ ATPase revealed an aberrant mitochondrial network in some ∆*atg9* parasites. Scale bar, 10 µm.

**Figure 7.. Autophagy is required for bradyzoite viability and the persistence of tissue cysts.**
Quantification of bradyzoite viability by quantitative polymerase chain reaction (qPCR)/plaque assay after differentiation media for 1 week followed by treatment with DMSO (vehicle control, blue) or LHVS (red) for a further 1 week (A) or 2 weeks (B). Data are from three biological replicates each with three technical replicates and are normalized to Pru∆*hxg* set at 100%. Bars represent mean ± SEM. (C) Viability of untreated bradyzoites after 2 weeks of differentiation in vitro. Each dot represents viability from one technical replicate. Data are merged from four biological replicates. Statistical comparisons were done using a Kruskal-Wallis test with Dunn’s multiple comparisons. Significance is indicated as ***p<0.001; ****p<0.0001. Non-significant differences are not indicated. (D) Analysis of virulence based on survival of infected mice. Mice were infected intraperitoneally with 150 tachyzoites of each strain. Infected mice that became moribund before the endpoint at day 35 post-infection were humanly euthanized. Mice infected with ∆*atg9* showed significantly better survival based on Mantel-Cox log-rank test (****p<0.0001). (E) Analysis of parasite dissemination to the brain. Brains were harvested from infected mice at 7 days post-infection and the number of genomes present in each brain homogenate was determined by qPCR. No significant differences were seen between strains based on analysis with a Kruskal-Wallis test with Dunn’s multiple comparisons. (F) Analysis of brain cyst burden in infected mice. Brains were harvested from mice 5 weeks post-infection and cysts were counted in blinded samples of brain homogenates by microscopy. Data is plotted as log₁₀ cysts per brain. The dotted line intersecting the y axis represents the limit of detection (<33 cysts/brain). Samples for which no cysts were observed in the 30 µl of homogenate analyzed were given a value that is half the limit of detection. Bars represent mean ± SEM and statistical comparisons were done using a Kruskal-Wallis test with Dunn’s multiple comparisons. Significance indicated as **p<0.01, ***p<0.001. Non-significant differences are not indicated.

**Figure 7—figure supplement 1.. Analysis of differentiation.**
In vitro parasitophorous vacuoles (PVs)/cysts were probed for the tachyzoite-specific marker SAG1 and the bradyzoite-specific marker BAG1. The intensity of SAG1 and BAG1 signals in each PV/cyst was determined using a pipeline in the automated image analysis software CellProfiler. The ratio of SAG1:BAG1 was calculated, log₂ transformed, and plotted. Each dot represents one technical replicate from three biological replicates. Statistical significance between samples was determined using a Kruskal-Wallis test with Dunn’s multiple comparisons and is indicated with ****p<0.0001 or ***p<0.001. Each biological replicate contained between 38 and 94 technical replicates. Each technical replicate represents an individual PV/cyst. A dotted line dissects the y axis at 0, indicating where SAG1 and BAG1 signal was equal and therefore data points below this line indicate PVs/cysts containing more BAG1 (bradyzoite marker) than SAG1 (tachyzoite marker).

**Figure 7—figure supplement 2.. TgATG9 is not required for tachyzoite plaque formation.**
Tachyzoites were isolated and applied to fresh cell monolayers for plaque formation over the course of 10 days. Plaques were normalized to 10³ genomes of input parasites, as measured by quantitative polymerase chain reaction (qPCR). Each dot represents one technical replicate from three (∆*atg9ATG9*) or four (Pru∆*hxg* and ∆*atg9*) biological replicates. No statistically significant differences were found using a Kruskal-Wallis test with Dunn’s multiple comparisons.

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Toxoplasma TgATG9 is critical for autophagy and long-term persistence in tissue cysts - PubMed

Toxoplasma TgATG9 is critical for autophagy and long-term persistence in tissue cysts

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