Statistical analysis The data were analyzed using SPSS Statistics 25 (IBM?) and GraphPad Prism 5.01 (GraphPad Software). humoral immune response against all known seasonal human coronaviruses including the new SARS\CoV\2, which could lead to a definition HS80 of low and high responders against human coronaviruses with potential impact on the assessment of postinfection antibody levels and protection. Keywords: humoral immune response, SARS\CoV\2, seasonal coronaviruses 1.?BACKGROUND At the end of December 2019, the first cases of severe pneumonia with an unknown cause were reported in Wuhan, China. HS80 1 , 2 The new virus is very similar to the beta\coronavirus SARS\coronavirus and was, therefore, named severe acute respiratory syndrome coronavirus 2 (SARS\CoV\2). SARS\CoV\2 is the cause of the current COVID\19 pandemic. 3 In addition to SARS\CoV\2, we know of six other human coronaviruses today. Among them are four seasonal human coronaviruses, that widely circulate in the human population and they are responsible for 10%C30% of moderate self\limiting upper respiratory tract infections. 4 A protective effect of previous infections with seasonal human coronaviruses against contamination with SARS\CoV\2 has been described as well as an association between previous infections with Rabbit polyclonal to ZNF10 seasonal human coronaviruses and less severe COVID\19 disease. 5 , 6 However, in first case the studies are based only on presumed infections due to the presence of clinical symptoms. In the latter case PCR confirmed HS80 infections with a seasonal human coronavirus are associated with less severe disease manifestations from SARS\CoV\2 contamination. To more clearly determine the effect of previous infections with human seasonal coronaviruses on the severity of disease and the humoral immune response to infections with SARS\CoV\2 we used enzyme\linked immunosorbent assay (ELISA) based immunoassays for the detection of antibodies against five different human coronaviruses and tested sera from SARS\CoV\2 convalescent plasma donors and a SARS\CoV\2 unexposed control group. 2.?PATIENTS AND METHODS 2.1. Study populace Characteristics of the study populace were summarized in Table?1. The study was approved by the local ethics committee al Heinrich\Heine University or college Duesseldorf (study no. 2020\1148). Informed consent was obtained from all of the SARS\CoV\2 convalescent plasma donors ((%)115 (100)114 (100)GenderMale (%)60 (52)67 (59)1.000Female (%)55 (48)47 (41)1.000Mean years (CI)44.5 (42.0C47.1)46.6 (44.1C49.2)0.252Median years (minCmax)47.9 (19.9C77.1)50.2 (20.3C77.9)Severity of disease (score) (%)05 (4)26.3 (?1.1C53.8)n.a.128 (24)47.0 (37.2C56.8)n.a.244 (38)53.9 (48.3C59.5)n.a.318 (16)51.0 (41.3C60.6)n.a.unclassified20 (17)Date of sampleMarchCJuly 2020MarchCJuly 2020 Open in a separate windows Abbreviation: CI, confidence interval. a The day after the onset of the disease when the blood sample was taken. 2.2. Enzyme\linked immunosorbent assay The detailed protocol for the anticoronavirus\N\protein GST capture ELISA was originally HS80 developed and recently published for the detection of antibodies against human polyoma computer virus JC and BK polyomaviruses. 7 , 8 Briefly, affinity\purified SARS\CoV\2, HCoV\HKU1, HCoV\OC43, HCoV\229E, and HCoV\NL63\Nucleocapsid (N) expressed as GST fusion proteins in BL21 cells in situ on gluthation casein\coated ELISA plates were used as antigens. RNA eluates from patient samples with PCR\confirmed coronavirus\infections of the University or college Hospital Dsseldorf were used for cloning the N genes with the exception of the N\gene of HCoV\HKU1, HS80 which was produced synthetically. To increase specificity, we chose a protocol in which cross\reactive antibodies are bound in a preincubation step with serum antibodies and a soluble heterologous coronavirus nucleocapsid protein. So, soluble SARS\CoV\2\N and HCoV\OC43\N bacterially expressed as fusion protein with N\terminal maltose\binding protein were generated for the pre\adsorption of all sera before the detection of the antibodies. For the SARS\CoV\2 assay, the sera were preadsorbed with soluble HCoV\OC43 N protein and for other assays with soluble SARS\CoV\2 N protein, respectively. Antigen\coated ELISA plates were incubated for 1?h with preadsorbed sera at 1:100 dilutions, and a polyclonal anti\human IgG peroxidase antibody (Sigma\Aldrich) and tetramethylbenzidine (BD Bioscience) were used for detection. The optical density (OD) was measured at 450?nm. The antibody reactivity were measured in arbitrary models (AU) and the dynamic range of the ELISAs were determined by serial dilution of human.