Impact of surfactant protein D, interleukin-5, and eosinophilia on Cryptococcosis.

Cryptococcus neoformans is an opportunistic fungal pathogen that initiates infection following inhalation. As a result, the pulmonary immune response provides a first line of defense against C. neoformans. Surfactant protein D (SP-D) is an important regulator of pulmonary immune responses and is typically host protective against bacterial and viral respiratory infections. However, SP-D is not protective against C. neoformans. This is evidenced by previous work from our laboratory demonstrating that SP-D-deficient mice infected with C. neoformans have a lower fungal burden and live longer than wild-type (WT) control animals. We hypothesized that SP-D alters susceptibility to C. neoformans by dysregulating the innate pulmonary immune response following infection. Thus, inflammatory cells and cytokines were compared in the bronchoalveolar lavage fluid from WT and SP-D(-/-) mice after C. neoformans infection. Postinfection, mice lacking SP-D have reduced eosinophil infiltration and interleukin-5 (IL-5) in lung lavage fluid. To further explore the interplay of SP-D, eosinophils, and IL-5, mice expressing altered levels of eosinophils and/or IL-5 were infected with C. neoformans to assess the role of these innate immune mediators. IL-5-overexpressing mice have increased pulmonary eosinophilia and are more susceptible to C. neoformans infection than WT mice. Furthermore, susceptibility of SP-D(-/-) mice to C. neoformans infection could be restored to the level of WT mice by increasing IL-5 and eosinophils by crossing the IL-5-overexpressing mice with SP-D(-/-) mice. Together, these studies support the conclusion that SP-D increases susceptibility to C. neoformans infection by promoting C. neoformans-driven pulmonary IL-5 and eosinophil infiltration.

Cryptococcus neoformans Rim101 is associated with cell wall remodeling and evasion of the host immune responses.

UNLABELLED: Infectious microorganisms often play a role in modulating the immune responses of their infected hosts. We demonstrate that Cryptococcus neoformans signals through the Rim101 transcription factor to regulate cell wall composition and the host-pathogen interface. In the absence of Rim101, C. neoformans exhibits an altered cell surface in response to host signals, generating an excessive and ineffective immune response that results in accelerated host death. This host immune response to the rim101Δ mutant strain is characterized by increased neutrophil influx into the infected lungs and an altered pattern of host cytokine expression compared to the response to wild-type cryptococcal infection. To identify genes associated with the observed phenotypes, we performed whole-genome RNA sequencing experiments under capsule-inducing conditions. We defined the downstream regulon of the Rim101 transcription factor and determined potential cell wall processes involved in the capsule attachment defects and altered mechanisms of virulence in the rim101Δ mutant. The cell wall generates structural stability for the cell and allows the attachment of surface molecules such as capsule polysaccharides. In turn, the capsule provides an effective mask for the immunogenic cell wall, shielding it from recognition by the host immune system. IMPORTANCE: Cryptococcus neoformans is an opportunistic human pathogen that is a significant cause of death in immunocompromised individuals. There are two major causes of death due to this pathogen: meningitis due to uncontrolled fungal proliferation in the brain in the face of a weakened immune system and immune reconstitution inflammatory syndrome characterized by an overactive immune response to subclinical levels of the pathogen. In this study, we examined how C. neoformans uses the conserved Rim101 transcription factor to specifically remodel the host-pathogen interface, thus regulating the host immune response. These studies explored the complex ways in which successful microbial pathogens induce phenotypes that ensure their own survival while simultaneously controlling the nature and degree of the associated host response.

Sterically crowded azulene-based dication salts as novel guests: synthesis and complexation studies with crown ethers and calixarenes in solution and in the gas phase.

The 1,4-bis(3-guaiazulenylmethylium)benzene and 1,4-bis[1-(4,6,8-trimethylazulenylmethylium)]benzene dication salts were synthesized via an acid-catalyzed condensation/dehydration protocol with guaiazulene-terephthalaldehyde (2 : 1 ratio), and 4,6,8-trimethylazulene-terephthalaldehyde (2 : 1 ratio) respectively in one-pot processes. A similar condensation reaction with the parent azulene led to an insoluble oligomer that was shown by MALDI-TOF-MS to contain 1,4-bis[(diazulenyl)methylium]benzene as a repeating unit. Dication salts and were fully characterized by 2D NMR and NOE techniques and by electrospray-MS (ES-MS) and MALDI-TOF-MS. NMR studies confirm that the dications are best represented as bis-tropylium species. A delicate balance of electronic (inductive stabilization) and steric influence of the alkyl groups on the seven-membered ring seems to influence the chemo-/regioselectivity of the co-condensation process. NMR titration and T(1) measurements established that, despite its highly crowded structure, dication forms host-guest HG complexes with dibenzo-30-crown-10 (DB30C10) and dibenzo-24-crown-8 (DB24C8) in solution, but fails to complex with the smaller dibenzo-18-crown-6 (DB18C6). The corresponding HG cation-molecule cluster ions were also detected in the gas phase by ES-MS, showing the formation of both dication-crown 1 : 1 and 1 : 2 complexes. Similar complexation of dication salt with DB30C10 was observed via NMR titration and T(1) measurements in solution and by ES-MS in the gas phase. Although solution complexation studies (NMR titration) did not indicate stable complex formation between and p-tert-butyl-methoxycalix[8]arene, their [HG](2+) and [H(2)G](2+) clusters were detectable by ES-MS. Solution decomplexation experiments (HG(2+) --> H + G(2+)) were performed on -crown complex by addition of DMSO, acetone, silver tosylate, and tropylium cation salt. Complexation of with DB30C10 was also studied by microcalorimetric titration.