Clinical Profile of SARS-CoV-2 Infection: Mechanisms of the Cellular Immune Response and Immunogenetic Markers in Patients from Brazil.

OBJECTIVES: The aim of this study is to evaluate some mechanisms of the immune response of people infected with SARS-CoV-2 in both acute infection and early and late convalescence phases. METHODS: This is a cohort study of 70 cases of COVID-19, confirmed by RT-PCR, followed up to 60 days. Plasma Samples and clinical data were. Viral load, blood count, indicators inflammation were the parameters evaluated. Cellular immune response was evaluated by flow cytometry and Luminex immunoassays. RESULTS: In the severe group, hypertension was the only reported comorbidity. Non severe patients have activated memory naive CD4+ T cells. Critically ill patients have central memory CD4+ T cell activation. Severe COVID-19 patients have both central memory and activated effector CD8+ T cells. Non-severe COVID-19 cases showed an increase in IL1ß, IL-6, IL-10 and TNF and severely ill patients had higher levels of the cytokines IL-6, IL-10 and CXCL8. CONCLUSIONS: The present work showed that different cellular responses are observed according to the COVID-19 severity in patients from Brazil an epicenter the pandemic in South America. Also, we notice that some cytokines can be used as predictive markers for the disease outcome, possibility implementation of strategies effective by health managers.

Zika Virus Infects Human Placental Mast Cells and the HMC-1 Cell Line, and Triggers Degranulation, Cytokine Release and Ultrastructural Changes.

Zika virus (ZIKV) is an emergent arthropod-borne virus whose outbreak in Brazil has brought major public health problems. Infected individuals have different symptoms, including rash and pruritus, which can be relieved by the administration of antiallergics. In the case of pregnant women, ZIKV can cross the placenta and infect the fetus leading to congenital defects. We have identified that mast cells in the placentae of patients who had Zika during pregnancy can be infected. This led to our investigation on the possible role of mast cells during a ZIKV infection, using the HMC-1 cell line. We analyzed their permissiveness to infection, release of mediators and ultrastructural changes. Flow cytometry detection of ZIKV-NS1 expression 24 h post infection in 45.3% of cells showed that HMC-1 cells are permissive to ZIKV infection. Following infection, ß-hexosaminidase was measured in the supernatant of the cells with a notable release at 30 min. In addition, an increase in TNF-α, IL-6, IL-10 and VEGF levels were measured at 6 h and 24 h post infection. Lastly, different intracellular changes were observed in an ultrastructural analysis of infected cells. Our findings suggest that mast cells may represent an important source of mediators that can activate other immune cell types during a ZIKV infection, which has the potential to be a major contributor in the spread of the virus in cases of vertical transmission.

Retention of a recombinant GFP protein expressed by the yellow fever 17D virus in the E/NS1 intergenic region in the endoplasmic reticulum.

The flaviviral envelope proteins, E protein and precursor membrane protein, are mainly associated with the endoplasmic reticulum (ER) through two transmembrane (TM) domains that are exposed to the luminal face of this compartment. Their retention is associated with the viral assembly process. ER-retrieval motifs were mapped at the carboxy terminus of these envelope proteins. A recombinant yellow fever (YF) 17D virus expressing the reporter green fluorescent protein (GFP) with the stem-anchor (SA) region of E protein fused to its carboxy terminus was subjected to distinct genetic mutations in the SA sequence to investigate their effect on ER retention. Initially, we introduced progressive deletions of the stem elements (H1, CS and H2). In a second set of mutants, the effect of a length increase for the first TM anchor region was evaluated either by replacing it with the longer TM of human LAMP-1 or by the insertion of the VALLLVA sequence into its carboxy terminus. We did not detect any effect on the GFP localisation in the cell, which remained associated with the ER. Further studies should be undertaken to elucidate the causes of the ER retention of recombinant proteins expressed at the intergenic E/NS1 region of the YF 17D virus polyprotein.

Retention of a recombinant GFP protein expressed by the yellow fever 17D virus in the E/NS1 intergenic region in the endoplasmic reticulum

The flaviviral envelope proteins, E protein and precursor membrane protein, are mainly associated with the endoplasmic reticulum (ER) through two transmembrane (TM) domains that are exposed to the luminal face of this compartment. Their retention is associated with the viral assembly process. ER-retrieval motifs were mapped at the carboxy terminus of these envelope proteins. A recombinant yellow fever (YF) 17D virus expressing the reporter green fluorescent protein (GFP) with the stem-anchor (SA) region of E protein fused to its carboxy terminus was subjected to distinct genetic mutations in the SA sequence to investigate their effect on ER retention. Initially, we introduced progressive deletions of the stem elements (H1, CS and H2). In a second set of mutants, the effect of a length increase for the first TM anchor region was evaluated either by replacing it with the longer TM of human LAMP-1 or by the insertion of the VALLLVA sequence into its carboxy terminus. We did not detect any effect on the GFP localisation in the cell, which remained associated with the ER. Further studies should be undertaken to elucidate the causes of the ER retention of recombinant proteins expressed at the intergenic E/NS1 region of the YF 17D virus polyprotein.

Aplicação de PCR em tempo real para avaliar viremia em humanos e primatas não humanos, imunizados com a vacina de febre amarela cepa 17DD e o vírus recombinante 17D-DENV / Application of PCR in real time to evaluate viremia in human beings and not human primates, immunized with the vaccine of yellow fever cepa 17DD and recombinant virus 17D-DENV

Um dos parâmetros principais para o estudo de atenuação de flavivírus é a determinação de sua capacidade de replicação. Neste contexto, empregamos o método de RT-PCR em tempo real que permite a detecção de ácidos nucléicos diretamente de amostras biológicas. Neste trabalho, utilizamos, então, esta tecnologia, para determinar a replicação de vírus de febre amarela 17DD e 17D-recombinantes, que expressam a proteína do envelope dos vírus dengue para validação destes como candidatos a vacinas. Esta metodologia foi empregada de forma complementar ao teste clássico de titulação viral por plaqueamento em culturas de células de vertebrados. Os materiais clínicos incluem soros de macacos rhesus previamente inoculados com estes vírus por via intracerebral ou subcutânea e soros de 32 indivíduos vacinados com vírus 17DD. O método demonstrou boa reprodutibilidade para amostras com título viral de até 2 Log10 PFU/mL com limite de detecção de até 10 PFU/mL ou 143 cópias /mL, sendo esta sensibilidade comparável ao que foi descrito para outros vírus analisados pela mesma tecnologia. Nesta faixa de concentração, os resultados obtidos pela metodologia de RT-PCR em tempo real mostraram-se compatíveis com os obtidos pelas técnicas de RT-PCR “semi nested” e pelo plaqueamento em soros de macacos inoculados com vírus 17DD. A análise comparativa da quantificação viral em espécimes clínicos de macacos sugere a limitada capacidade de replicação do vírus 17DD independente da via de inoculação. Os vírus 17D-recombinantes, avaliados neste estudo, demonstraram sua atenuação em relação ao vírus 17DD, tanto pela metodologia de RT-PCR em tempo real como por plaqueamento. Assim sendo, consideramos que a tecnologia empregada para o estudo da capacidade replicativa dos vírus 17DD e 17D-recombinantes em diferentes hospedeiros, demonstrou o perfil de atenuação dos vírus testados. Com relação aos vírus recombinantes 17D-dengue, estes resultados embasam a continuação do seu desenvolvimento como cand...