Abstract
Pneumocystis pneumonia is the most common serious opportunistic infection in patients with HIV/AIDS. Furthermore, Pneumocystis pneumonia is a feared complication of the immunosuppressive drug regimens used to treat autoimmunity, malignancy, and posttransplantation rejection. With an increasing at-risk population, there is a strong need for novel approaches to discover diagnostic and vaccine targets. There are multiple challenges to finding these targets, however. First, Pneumocystis has a largely unannotated genome. To address this, we evaluated each protein encoded within the Pneumocystis genome by comparisons to proteins encoded within the genomes of other fungi using NCBI BLAST. Second, Pneumocystis relies on a multiphasic life cycle, as both the transmissible form (the ascus) and the replicative form (the trophozoite [troph]) reside within the alveolar space of the host. To that end, we purified asci and trophs from Pneumocystis murina and utilized transcriptomics to identify differentially regulated genes. Two such genes, Arp9 and Sp, are differentially regulated in the ascus and the troph, respectively, and can be utilized to characterize the state of the Pneumocystis life cycle in vivoGsc1, encoding a β-1,3-glucan synthase with a large extracellular domain previously identified using surface proteomics, was more highly expressed on the ascus form of Pneumocystis GSC-1 ectodomain immunization generated a strong antibody response that demonstrated the ability to recognize the surface of the Pneumocystis asci. GSC-1 ectodomain immunization was also capable of reducing ascus burden following primary challenge with Pneumocystis murina Finally, mice immunized with the GSC-1 ectodomain had limited fungal burden following natural transmission of Pneumocystis using a cohousing model.IMPORTANCE The current report enhances our understanding of Pneumocystis biology in a number of ways. First, the current study provided a preliminary annotation of the Pneumocystis murina genome, addressing a long-standing issue in the field. Second, this study validated two novel transcripts enriched in the two predominant life forms of Pneumocystis These findings allow better characterization of the Pneumocystis life cycle in vivo and could be valuable diagnostic tools. Furthermore, this study outlined a novel pipeline of -omics techniques capable of revealing novel antigens (e.g., GSC-1) for the development of vaccines against Pneumocystis.
Highlights
Pneumocystis pneumonia is the most common serious opportunistic infection in patients with HIV/AIDS
Expression is shown as the log2 of troph expression divided by ascus expression. (D) Genes with significantly differential expression as measured by a t test performed with Benjamini and Hochberg correction (P Ͻ 0.005). (E) Genes expressed only in the ascus (n ϭ 123) or troph (n ϭ 20) as filtered by a quality value of 10. (F) A putative extracellular serine protease showed increased expression in the troph (P Ͻ 0.001). (G) A putative RNA-induced silencing complex (RISC) subunit, Arp9, showed increased expression in the ascus (P Ͻ 0.001). (H) Differential levels of RNA expression of the seven genes previously identified via surface proteomics (*, P Ͻ 0.05; **, P Ͻ 0.01)
Pneumocystis utilizes a multiphasic life cycle involving the propagation of asci and trophs within the alveolar space of the host [19, 27]
Summary
Pneumocystis pneumonia is the most common serious opportunistic infection in patients with HIV/AIDS. Pneumocystis relies on a multiphasic life cycle, as both the transmissible form (the ascus) and the replicative form (the trophozoite [troph]) reside within the alveolar space of the host. GSC-1 ectodomain immunization generated a strong antibody response that demonstrated the ability to recognize the surface of the Pneumocystis asci. GSC-1 ectodomain immunization was capable of reducing ascus burden following primary challenge with Pneumocystis murina. This study validated two novel transcripts enriched in the two predominant life forms of Pneumocystis. These findings allow better characterization of the Pneumocystis life cycle in vivo and could be valuable diagnostic tools. The fluidity of the Pneumocystis life cycle can present a challenge for diagnosis, as at least one case of GMS-negative Pneumocystis has been described previously [28]
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