Zi T. Wang’s research while affiliated with Washington University in St. Louis and other places

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Publications (13)

Supplementary Material
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August 2018

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21 Reads

Gabriel R. de Abreu Cabral

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Zi T. Wang

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Nitric oxide (NO) production (nitrite in μM) in activated J774-A1 and RAW 264.7 cells macrophages after T. gondii infection. (A) NO production of non-infected (Control) or T. gondii (RH) infected J774-A1cells at 6 h and (B) 24 h post-infection. Mean ± SEM (n = 3 experiments, each with 12 replicates). (C) NO production of non-infected (Control) or T. gondii (RH) infected RAW 264.7 cells at 6 h and (D) 24 h post-infection. Mean ± SEM (n = 3 experiments, each with 12 replicates). ns (not significant), ∗P ≤ 0.05, ∗∗P ≤ 0.01, ∗∗∗P ≤ 0.001, two-way ANOVA with Tukey post-test. (E) NO production of non-infected (Control) or T. gondii (RH) infected J774-A1 (F) or RAW 264.7 cells for 24 h with normal medium or supplemented with different levels of L-arginine. Mean ± SEM (n = 3 experiments, each with 6 replicates). ∗P ≤ 0.05 and ∗∗P ≤ 0.01, ∗∗P ≤ 0.01, ∗∗∗P ≤ 0.001, ∗∗∗∗P ≤ 0.0001 one-way ANOVA with Tukey post-test, #P ≤ 0.05 comparing the “Control” or “Infected” bar with the respective “Normal medium” bar.
Immunofluorescence detection of iNOS in activated J774-A1 macrophages infected with T. gondii. (A) Detection of iNOS (green) in non-infected (Control) and in T. gondii (red) infected cells (DAPI - blue) at 2, 6, and 24 h post-infection. Scale bar = 10 μm. (B) Analysis of the proportion of iNOS positive or negative macrophages in non-infected (Control) and T. gondii infected cells at 2 and 24 h post-infection. Mean ± SEM (n = 4 experiments, each with 8 replicates). (C) Western blot detection of iNOS expression in non-infected (Control) and T. gondii infected (Infected) cells. β-actin was used as loading control. (D) Densitometry of western blots normalized to β-actin at 2 h post-infection. Mean ± SD (n = 3 experiments, each with 1 replicate). ∗P ≤ 0.05, two-way ANOVA with Tukey post-test, n.s (not significant).
Immunofluorescence detection of iNOS in activated RAW 264.7 macrophages infected with T. gondii. (A) Detection of iNOS (green) in non-infected (Control) and in T. gondii (red) infected cells (DAPI - blue) at 2, 6, and 24 h post-infection. Scale bar - 10 μm. (B) Analysis of the proportion of iNOS positive or negative macrophages in non-infected (Control) and T. gondii infected cells at 2 and 24 h post-infection. Mean ± SEM (n = 4 experiments, each with 8 replicates). (C) Western blot detection of iNOS expression in non-infected (Control) and T. gondii - infected (Infected) cells at different time intervals post-infection. β-actin was used as loading control. (D) Densitometry of western bolts normalized to β-actin at 2 h post-infection. Mean ± SD (n = 3 experiments, each with 1 replicate), n.s (not significant).
Analysis of ROP and ASP5, MYR1, and IST deletion mutants on the ability of T. gondii to inhibit NO production (nitrite in μM) of activated macrophages. (A) NO production of non-infected (Control) or activated J774-A1 cells infected with parental (RHΔku80 strain) or various ROP deletion strains of T. gondii at 24 h post-infection. Mean ± SEM (n = 3 experiments, each with 12 replicates). ∗∗∗∗P ≤ 0.0001, one-way ANOVA with Tukey post-test. (B) NO production of non-infected (Control) or activated J774-A1 cells infected with parental (RHΔku80 strain) or Δasp5, Δmyr1, or Δist mutant strains of T. gondii at 24 h post-infection. Mean ± SEM (n = 3 experiments, each with 12 replicates). ∗∗∗∗P ≤ 0.0001, one-way ANOVA with Tukey post-test. (C) NO production of non-infected (Control) or activated RAW 264.7 cells infected with parental (RHΔku80 strain) or various ROP deletion strains of T. gondii at 24 h post-infection. Mean ± SEM (n = 3 experiments, each with 12 replicates). ∗P ≤ 0.05, ∗∗P ≤ 0.01, ∗∗∗P ≤ 0.001, ∗∗∗∗P ≤ 0.0001, one-way ANOVA with Tukey post-test. (D) NO production of non-infected (Control) or activated RAW 264.7 cells infected with parental (RHΔku80 strain) or Δasp5, Δmyr1, and Δist mutant strains of T. gondii at 24 h post-infection. Mean ± SEM (n = 3 experiments, each with 12 replicates). ∗P ≤ 0.05, ∗∗P ≤ 0.01, one-way ANOVA with Tukey post-test.
Inhibition of Nitric Oxide Production in Activated Macrophages Caused by Toxoplasma gondii Infection Occurs by Distinct Mechanisms in Different Mouse Macrophage Cell Lines

August 2018

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840 Reads

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31 Citations

Gabriel R. de Abreu Cabral

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Zi T. Wang

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Toxoplasma gondii, the causative agent of toxoplasmosis, is a widespread intracellular parasite able to infect virtually any nucleated cell. T. gondii infection of activated macrophages inhibits nitric oxide (NO) production; however, parasite effectors responsible for this block have not been defined. Macrophage populations are extremely heterogeneous, responding differently to stimuli and to parasite infection. Here we evaluated the inhibition of NO production caused by T. gondii infection of J774-A1 and RAW 264.7 macrophages and assessed the role of several known parasite virulence factors in this phenotype. Infection of activated macrophages from both macrophage lines reduced NO production, however, the mechanism of this decrease was different. Consistent with previous reports, infected J774-A1 macrophages had reduced iNOS expression and lower number of iNOS positive cells. In contrast, T. gondii infection of RAW 264.7 macrophages did not alter iNOS expression or the number of iNOS positive cells, and yet it led to lower levels of NO production. Deletion of a number of previously defined virulence factors including ROP kinases that disrupt innate immune factors, TgIST which blocks STAT1 activation, as well as the secretory trafficking proteins ASP5 and MYR1, did not alter the phenotype of decreased NO production. Taken together our findings indicate that T. gondii infection inhibits NO production of activated macrophages by different mechanisms that involve reduction of iNOS expression vs. iNOS impairment, and suggest that a novel parasite effector is involved in modulating this important host defense pathway.

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AAH2 gene is not required for dopamine-dependent neurochemical and behavioral abnormalities produced by Toxoplasma infection in mouse

March 2018

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58 Reads

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31 Citations

Behavioural Brain Research

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Zi Teng Wang

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Infection with the protozoan parasite, Toxoplasma gondii (T. gondii), has been associated with the increased risk for several psychiatric disorders. The exact mechanisms of a hypothesized contribution of T. gondii infection are poorly understood. The T. gondii genome contains two aromatic amino acid hydroxylase genes (AAH1 and AAH2) that encode proteins that can produce L-DOPA. One popular hypothesis posits that these encoded enzymes might influence dopamine (DA) production and hence DA synaptic transmission, leading to neurobehavioral abnormalities in the infected host. Prior studies have shown that deletion of these genes does not alter DA levels in the brain or exploratory activity in infected mice. However, possible effects of AAH gene deficiency on infection-induced brain and behavior alterations that are directly linked to DA synaptic transmission have not been evaluated. We found that chronic T. gondii infection of BALB/c mice leads to blunted response to amphetamine or cocaine and decreased expression of Dopamine Transporter (DAT) and Vesicular Monoamine Transporter 2 (VMAT2). Deletion of AAH2 had no effects on these changes in infected mice. Both wild type and Δaah2 strains produced comparable levels of neuroinflammation. Our findings demonstrate that AAH2 is not required for T. gondii infection-produced DA-dependent neurobehavioral abnormalities.

Copy number analysis of AAH2 in T. gondii strains (A) Copy number variation (CNV) of Tg_ME49_212740 (AAH2) in five representative strains. (B) CNV at each base across the AAH2 gene in ME49. Red lines indicate the start and stop codons of AAH2. (C) PCR using primers (Z28+ Z65) (S3 Table) common to both AAH1 and AAH2 were used against the ME49 genome to amplify both genes for Sanger sequencing and single nucleotide polymorphism (SNP) determination. (D) Sanger sequencing of PCR fragments against the AAH genes of the wild type ME49 Δhxg::Luc strain shows a 2:1 ratio of AAH2 to AAH1 SNPs, indicating a duplication of the AAH2 gene. Each SNP in the chromatograph is marked by a red dot. In the Δaah2::HXG knockout, all AAH2 SNPs are no longer visible, indicating loss of both copies of the AAH2 gene.
Disruption of the AAH1 and AAH2 genes (A) Schematic of the AAH2 knockout strategy in the wild-type ME49 Δhxg::Luc strain (referred to as WT). A CRISPR-Cas9 construct with guide RNAs targeted to the 5’ and 3’ UTRs of AAH2 was co-transfected with the pΔaah2::HXG plasmid (S2 Table) and selected for with MPA +Xanthine to delete AAH2 to produce the clone Δaah2::HXG (Δh2-HXG). Subsequently, the HXG gene was replaced with either a clean fusion of the AAH2 5’ and 3’ UTRs (pΔaah2) or an AAH2 cDNA construct (pAAH2). (S2 Table) using 6-thioxanthine selection against the HXG locus to create the clean knockout clone Δaah2 (Δh2) (upper panel) and the complement clone Δaah2::AAH2 (Δh2-H2) (lower panel). Yellow Bars: CRISPR targeting sites. Black bars: PCR screening primer target regions (S3 Table). (B) Schematic of the knockout strategy for AAH1. A CRISPR-Cas9 construct with guide RNAs targeted to the 5’ and 3’ UTRs of AAH1 was co-transfected with the pΔaah1::DHFR-Ts repair construct (S2 Table) into WT or Δaah2 parasites to create the clones Δaah1 (Δh1) and Δaah1Δaah2 (Δh1Δh2). Transfectants were selected for via pyrimethamine resistance. Subsequently, using pΔuprt::AAH1::HXG, a cDNA copy of AAH1 driven by its native 5’ and 3’ UTRs was complemented into the UPRT locus by means of the HXGPRT drug resistance marker selected for with MPA +Xanthine, negative selection against UPRT with FUDR, and a single-cutting CRISPR-Cas9 construct targeted to the UPRT gene (S2 Table), creating the complement clones Δaah1-AAH1 (Δh1-H1) and Δaah1Δaah2-AAH1 (Δh1Δh2-H1). Brown & Yellow Bars: CRISPR targeting sites. Black bars: PCR screening primer target regions (S3 Table). (C) PCR verification of successful ablation and complementation of knockouts. Expected product sizes: Tubulin (Tub): 0.378kb. AAH1 (H1): 0.745kb (Native), 0.278kb (cDNA). AAH2 (H2): 0.745kb (Native), 0.278kb (cDNA). (D) Growth assays of parasites seeded into 96-well plates and allowed to proliferate for 24 h, then quantified using a luciferase assay. The WT, Δh1, Δh2, Δh1Δh2, Δh1-H1, Δh2-H2, and Δh1Δh2-H1 parasites showed no significant difference in total growth (Kruskal-Wallis test, P = 0.0672, N = 3 per strain).
Development of bradyzoites in vitro and in vivo (A) There was no significant difference in bradyzoite differentiation in vitro across the parasite lines in either tachyzoite conditions (left) (P> 0.99) or bradyzoite conditions (right) (P> 0.99) (Two-way ANOVA).(B) Representative pictures of tachyzoites, partial cysts, and complete cysts produced in vitro as assessed by DBL staining. (C) Brain cyst yields in mice 1–2 months post-infection. All parasite lines produced similar numbers of tissue cysts in vivo (Kruskal-Wallis, ns).
Development of oocysts following infection of cats (A) Yields of oocysts shed from infected cats. The yield of knockout mutants as a whole were significantly reduced relative to the wild-type (Kruskal-Wallis, P ≤0.05), however due to low sample size, pairwise comparisons between each mutant and the WT approached, but did not reach significance (Δh1 P = 0.116, Δh2 P = 0.821, Δh1Δh2 P = 0.116). (B) The sporulation success rate of shed oocysts shows a significant defect in mutant lines (Dunn’s multiple comparisons test, for wild type vs. Δh2 P = 0.0008; and for the wild type vs. Δh1-H1 P = 0.0178 and Δh1Δh2-H1 P< 0.0001). The oocyst yields of Δh1 and Δh1Δh2 parasites were not sufficient to allow quantification (not done = N.D.). Each result is displayed as the Mean ±SD of three replicate counts of oocysts (n ≥ 50 per count) from one cat.
Representative fluorescence microscope images of dityrosine autofluorescence in sporulated and unsporulated oocysts of WT, Δh1, Δh2, and Δh1Δh2 oocysts All images were taken at 1000-1600ms exposure using a DAPI UV filter, but due to rapid photobleaching and differing levels of background signal in different oocyst fecal suspensions, direct comparison and quantification of fluorescence is not feasible. Scale bar = 10μm.

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The aromatic amino acid hydroxylase genes AAH1 and AAH2 in Toxoplasma gondii contribute to transmission in the cat

March 2017

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232 Reads

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39 Citations

Zi T. Wang

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Jitender P. Dubey

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The Toxoplasma gondii genome contains two aromatic amino acid hydroxylase genes, AAH1 and AAH2 encode proteins that produce L-DOPA, which can serve as a precursor of catecholamine neurotransmitters. It has been suggested that this pathway elevates host dopamine levels thus making infected rodents less fearful of their definitive Felidae hosts. However, L-DOPA is also a structural precursor of melanins, secondary quinones, and dityrosine protein crosslinks, which are produced by many species. For example, dityrosine crosslinks are abundant in the oocyst walls of Eimeria and T. gondii, although their structural role has not been demonstrated, Here, we investigated the biology of AAH knockout parasites in the sexual reproductive cycle within cats. We found that ablation of the AAH genes resulted in reduced infection in the cat, lower oocyst yields, and decreased rates of sporulation. Our findings suggest that the AAH genes play a predominant role during infection in the gut of the definitive feline host.

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Generation of an AAH2-deficient strain and genetic complementation. (A) Schematic of AAH2 knockout strategy. (Left) HXGPRT construct flanked by 5′ and 3′ regions from the AAH2 genomic locus was used to knock out the AAH2 gene in the PruΔku80Δhxg background by double homologous crossover. MPA, mycophenolic acid; Xa, xanthine, which was used for selection. (Center) The deletion strain (Δaah2::HXG) was transfected with cleanup construct to remove the HXGPRT drug marker. (Right) The deletion strain (Δaah2::HXG) was complemented by replacing HXGPRT with a cDNA copy of AAH2. (B) Diagnostic PCR of the wild-type (PruΔku80Δhxg), deletion mutant (PruΔku80ΔhxgΔaah2), and complement (PruΔku80ΔhxgΔaah2::AAH2) lines. Arrows show the respective primers used to confirm the genetic architecture (see Table S1 in the supplemental material). Expected product sizes were the following: AAH1, 4.820 kb; AAH2, 4.820 kb; AAH2 cDNA, 1.698 kb. (C) Plaque assay measuring in vitro growth of strains on HFF monolayers stained with crystal violet.
Differentiation into bradyzoites in vitro. (A) Formation of cysts by wild-type, Δaah2, and Δaah2::AAH2 parasites in tachyzoite and bradyzoite conditions in vitro. Partial and fully formed cysts were enumerated based on staining with DBL. There was no significant difference in cyst formation in bradyzoite-induced parasites (P = 1.00) and no significant difference in cyst formation (P = 0.66) or partial cyst formation (P = 0.88) in tachyzoite conditions (both determined by one-way ANOVA; n = 3 experiments). (B) Representative pictures of intact, partial, and absent cyst formation in parasite vacuoles. Blue, 4′,6-diamidino-2-phenylindole (DAPI); red, GRA7; green, DBL. Scale bar, 10 μm.
Differentiation and expression levels in tachyzoites and bradyzoites. (A) Quantitative real-time PCR comparing gene expression of bradyzoites relative to that of tachyzoites of wild-type, knockout (Δaah2), and complemented (Δaah2::AAH2) parasites. Stage-specific markers SAG1, BAG1, SAG2A, and LDH2, along with AAH1 and AAH2, were monitored with gene-specific primers (see Table S1 in the supplemental material). Results are means ± standard deviations (SD) (n = 3 experiments). Excluding the expected differences in AAH2 expression, expression differences between the genes probed were not significant (P = 0.19 by two-way ANOVA). (B) Western blot of bradyzoites expressing a Ty epitope-tagged AAH1 or AAH2 or a tagged copy of AAH2 driven by the BAG1 promoter. Red, GRA2; green, Ty. Expected protein sizes: AAH1 and AAH2, 55 kDa; GRA2 (dense granule protein 2), 28 kDa. (C) Immunofluorescent assay of AAH1-Ty-, AAH2-Ty-, and BAG1::H2Ty-tagged parasites differentiated into bradyzoites. Blue, DAPI; green, DBL; red, Ty. Scale bar, 10 μm.
Production of dopamine in infected PC12 cells. (A) Comparison of infection with wild-type, knockout (Δaah2), complement (Δaah2::AAH2), or BAG1-2Ty overexpressor tachyzoites in PC12 cells (P = 0.40 by one-way ANOVA). Results are means ± SD (n = 2 to 5 replicates). The y axis shows the ratio of dopamine content per PC12 cell relative to uninfected PC12s. (B) Comparison of dopamine content in PC12 cells grown under bradyzoite conditions (P = 0.4239 by one-way ANOVA). Results are means ± SD (n = 2 to 4).
Dopamine content in the brain of control and infected mice. (A) Parasite cyst burden in whole brains of CD1 mice examined at 1 (1 mo) or 2 months (2 mo) postinfection. Infection with ME49 at 1 mo showed significantly higher cyst burden (P = 0.0003 by Kruskal-Wallis test with Dunn's multiple comparisons for Pru strains and ME49). Infection with the type III C56 strain showed significantly lower cyst burden (P = 0.0003 by Kruskal-Wallis test with Dunn's multiple comparisons for Pru strains and C56), with 5 of 10 mice showing cyst burdens below the detectable limit of 20 cysts/brain (not plotted). (B) Dopamine levels in total brain homogenates in uninfected and infected mice at 1 (1mo) or 2 (2mo) months postinfection. Dopamine levels were not significantly different between infected or uninfected animals or between infection strains (P = 0.075 by Kruskal-Wallis test with Dunn's multiple comparisons test). (C) Linear regression analysis between cyst density and brain dopamine concentration in mice infected with ME49 for 1 month (1mo) or 2 months (2mo). R² = 0.1333 (red). If the highest point in the linear regression was removed, R² = 0.1175 (blue).
Reassessment of the Role of Aromatic Amino Acid Hydroxylases and the Effect of Infection by Toxoplasma gondii on Host Dopamine

February 2015

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32 Reads

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70 Citations

Zi T. Wang

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Steve Harmon

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Karen L. O'Malley

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Toxoplasma gondii infection has previously been described to cause infected mice to lose their fear of cat urine. This behavioral manipulation has been proposed to involve alterations of host dopamine pathways due to parasite-encoded aromatic amino acid hydroxylases. Here, we report successful knockout and complementation of the aromatic amino acid hydroxylase AAH2 gene, with no observable phenotype in parasite growth or differentiation in vitro and in vivo. Additionally, expression levels of the two aromatic amino acid hydroxylases were negligible both in tachyzoites and in bradyzoites. Finally, we were unable to confirm previously described effects of parasite infection on host dopamine either in vitro or in vivo, even when AAH2 was over-expressed using the BAG1 promoter. Together, these data indicate that AAH enzymes in the parasite do not cause global or regional alterations of dopamine in the host brain, although they may locally affect this pathway. Additionally, our findings suggest alternative roles for the AHH enzymes in T. gondii since AAH1 is essential for growth in non-dopaminergic cells. Copyright © 2014, American Society for Microbiology. All Rights Reserved.

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Citations (7)

... In addition, skeletal muscle cells treated with IFNγ and TNF have been shown to recruit IRGb6 to the vacuole and produce nitrite in response to Type I and Type II parasite infection; however, a direct relationship between these effector mechanisms was not tested 63 . Perhaps the most critical evidence supporting the importance of iNOS in T. gondii clearance is the observation that parasites have evolved strategies to inhibit the • NO production 64,65 and promote the proteasomal degradation of iNOS 64 . The Knoll lab found that T. gondii patatinlike protein (TgPL1) limited nitrite synthesis in LPS and IFNγ-stimulated macrophages and protected parasites from degradation 66,67 , however, the precise mechanism by which TgPL1 interrupts the iNOS/ • NO axis is not clear. ...

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iNOS is necessary for GBP-mediated T. gondii clearance in murine macrophages via vacuole nitration and intravacuolar network collapse
Inhibition of Nitric Oxide Production in Activated Macrophages Caused by Toxoplasma gondii Infection Occurs by Distinct Mechanisms in Different Mouse Macrophage Cell Lines
Gabriel R. de Abreu Cabral

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Zi T. Wang

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... T. gondii infection promotes dopamine release in neurons, most likely by self-expression of genes encoding the rate-limiting enzyme for dopamine synthesis [8,9]. The parasite also disrupts glutamate signaling in the brain by interfering with the kynurenine pathway [10]. ...

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Toxoplasmosis in Patients with Psychosis: A Cross-Sectional Study
AAH2 gene is not required for dopamine-dependent neurochemical and behavioral abnormalities produced by Toxoplasma infection in mouse
  • Citing Article

  • March 2018

Behavioural Brain Research

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Zi Teng Wang

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... Phenylalanine, tyrosine and tryptophan biosynthesis pathway are essential for the infection of T. gondii in cats. A previous study showed that the knock-out of AAH1 and AAH2 in T. gondii can reduce T. gondii infection in cats, lower oocyst yields, and decrease sporulation rates [79]. AAH1 and AAH2 of T. gondii can catalyse the conversion of phenylalanine to tyrosine, and then convert tyrosine to 3,4 dihydroxyphenylalanine (L-DOPA) [80], which is critical for the survival of T. gondii [81]. ...

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Dynamic RNA profiles in the small intestinal epithelia of cats after Toxoplasma gondii infection
The aromatic amino acid hydroxylase genes AAH1 and AAH2 in Toxoplasma gondii contribute to transmission in the cat
Zi T. Wang

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Jitender P. Dubey

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... This result is consistent with previous studies and with already known neurobiological mechanisms (2,4). Studies of mammals have shown that a chronic infection with T. gondii affects the regulation of neurotransmitters and in particular dopamine metabolism (4). ...

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Additional Clinical Aspects
Reply to “Reproducing Increased Dopamine with Infection To Evaluate the Role of Parasite-Encoded Tyrosine Hydroxylase Activity”
Zi Teng Wang

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... It is interesting that the dopamine transporters Slc35f3 and Slc17a6 were 1.8-fold and 1.9-fold more abundant, respectively. Several research groups have previously seen a connection between T. gondii infection dopamine metabolism as well as host behavior (68)(69)(70)(71)(72). Perhaps, RNASeq at an earlier infection time point would capture greater differences in these dopamine transporters. ...

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Toxoplasmosis accelerates the progression of hereditary spastic paraplegia
Reassessment of the Role of Aromatic Amino Acid Hydroxylases and the Effect of Infection by Toxoplasma gondii on Host Dopamine
Zi T. Wang

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Steve Harmon

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Karen L. O'Malley

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... Sortmerna v4.3.4 (72) was used to remove any rRNA reads. The remaining reads were aligned to either the published MBIC11017 reference genome (73) or the MU13 draft genome assembly (24) using bowtie2 v2.3.4.3 (74). Reads were counted for CDS, tRNA, and pseudogene features using htseq-count v2.0.2 (75). ...

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Integration of horizontally acquired light-harvesting genes into an ancestral regulatory network in the cyanobacterium Acaryochloris marina MBIC11017
Niche adaptation and genome expansion in the chlorophyll d-producing cyanobacterium Acaryochloris marina

Proceedings of the National Academy of Sciences

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Patricia C Cheung

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... Strong irreversible binding of NEM to thiols may stop the proper functioning of cytosolic low molecular mass (LMM) redox buffers like free cysteine, glutathione [56] and bacillithiols, which H. modesticaldum uses in lieu of glutathione [63]. Upon entering the cytosol, Hg II will likely interact with intracellular thiol-based redox buffers such as bacillithiols and free cysteines and quench or possibly oxidize them [64,65]. ...

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Anaerobic HgII reduction is driven by cellular HgII-thiol interactions
The Genome of Heliobacterium modesticaldum, a Phototrophic Representative of the Firmicutes Containing the Simplest Photosynthetic Apparatus

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