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      Characterization of the Humoral Immune Response to Porcine Epidemic Diarrhea Virus Infection under Experimental and Field Conditions Using an AlphaLISA Platform

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          Abstract

          Coronavirus infections are a continuous threat raised time and again. With the recent emergence of novel virulent strains, these viruses can have a large impact on human and animal health. Porcine epidemic diarrhea (PED) is considered to be a reemerging pig disease caused by the enteropathogenic alphacoronavirus PED virus (PEDV). In the absence of effective vaccines, infection prevention and control through diagnostic testing and quarantine are critical. Early detection and differential diagnosis of PEDV infections increase the chance of successful control of the disease. Therefore, there is a continuous need for development of reduced assay-step protocols, no-wash, high-throughput immunoassays. This study described the characterization of the humoral immune response against PEDV under experimental and field conditions using a rapid, sensitive, luminescent proximity homogenous assay (AlphaLISA). PEDV IgG and IgA antibodies were developed toward the beginning of the second week of infection. PEDV IgG antibodies were detected for at least 16 weeks post-exposure. Remarkably, the serum IgA levels remained high and relatively stable throughout the study, lasting longer than the serum IgG response. Overall, AlphaLISA allows the detection and characterization of pathogen-specific antibodies with new speed, sensitivity, and simplicity of use. Particularly, the bridge assay constitutes a rapid diagnostic that substantially improves upon the “time to result” metric of currently available immunoassays.

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          A new coronavirus-like particle associated with diarrhea in swine

          Summary Coronavirus-like particles were detected by electron microscopy in the intestinal contents of pigs during a diarrheal outbreak on 4 swine breeding farms. Diarrhea was reproduced in experimental pigs with one of the isolates, designated CV777, which was found to be distinct from the 2 known porcine coronaviruses, transmissible gastroenteritis virus and hemagglutinating encephalomyelitis virus.
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            Emergence of Porcine epidemic diarrhea virus in the United States: clinical signs, lesions, and viral genomic sequences.

            During the 10 days commencing April 29, 2013, the Iowa State University Veterinary Diagnostic Laboratory received the first 4 of many submissions from swine farms experiencing explosive epidemics of diarrhea and vomiting affecting all ages, with 90-95% mortality in suckling pigs. Histology revealed severe atrophy of villi in all segments of the small intestines with occasional villus-epithelial syncytial cells, but testing for rotaviruses and Transmissible gastroenteritis virus (Alphacoronavirus 1) were negative. Negative-staining electron microscopy of feces revealed coronavirus-like particles and a pan-coronavirus polymerase chain reaction (PCR) designed to amplify a conserved region of the polymerase gene for all members in the family Coronaviridae produced expected 251-bp amplicons. Subsequent sequencing and analysis revealed 99.6-100% identity among the PCR amplicons from the 4 farms and 97-99% identity to the corresponding portion of the polymerase gene of Porcine epidemic diarrhea virus (PEDV) strains, with the highest identity (99%) to strains from China in 2012. Findings were corroborated at National Veterinary Services Laboratories using 2 nested S-gene and 1 nested N-gene PCR tests where the sequenced amplicons also had the highest identity with 2012 China strains. Whole genome sequence for the virus from 2 farms in 2 different states using next-generation sequencing technique was compared to PEDV sequences available in GenBank. The 2013 U.S. PEDV had 96.6-99.5% identity with all known PEDV strains and the highest identity (>99.0%) to some of the 2011-2012 Chinese strains. The nearly simultaneous outbreaks of disease, and high degree of homology (99.6-100%) between the PEDV strains from the 4 unrelated farms, suggests a common source of virus.
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              Outbreak of Porcine Epidemic Diarrhea in Suckling Piglets, China

              To the Editor: Beginning in October 2010, porcine epidemic diarrhea (PED), caused by a coronaviral infection affecting pigs, emerged in China in an outbreak characterized by high mortality rates among suckling piglets. The outbreak overwhelmed >10 provinces in southern China, and >1,000,000 piglets died. This outbreak was distinguished by ≈100% illness among piglets after birth (predominantly within 7 days and sometimes within only a few hours) and death rates of 80%–100% (Technical Appendix Table 1). Few sows or boars showed any clinical signs during the outbreak, which is not consistent with a recent report from Thailand ( 1 ). In that outbreak during late 2007, pigs of all ages were affected, exhibiting different degrees of diarrhea and no appetite. We characterized the genetic variation of the PED virus (PEDV) that caused a large-scale outbreak in China during 2010–2011 and compared it with viruses in other outbreaks. We also report a possible novel transmission pathway for PEDV. A total of 177 samples (intestine, stool, and maternal milk) were collected from pigs from different farms who had diarrhea; 100% of farms had >1 porcine sample positive for PEDV. A total of 125/177 porcine samples were confirmed as positive for PEDV by reverse transcription PCR using primers as described ( 2 ). PEDV was detected in 105 (82.0%) of 128 fecal samples and 20 (40.8%) of 49 sow milk samples. Piglets infected with PEDV showed mild hemorrhage, undigested curdled milk in the stomach, and thin-walled intestines with severe mucosal atrophy and foamy fluid (data not shown). The spike (S) gene of the family Coronaviridae has a high degree of variation and can induce neutralizing antibody ( 3 ). Reverse transcription PCR products of the 651-bp partial S gene of PEDV and the deduced amino acid sequences were aligned by using ClustalW (www.genome.jp/tools/clustalw), and a neighbor-joining tree with 1,000 bootstraps was constructed. Sequences of the S genes from this outbreak were 99.1%–100.0% homologous and had 88.7%–98.9% nt identity with all reference strains (Technical Appendix Table 2), 98.5%–98.9% with Thailand strains, and 94.5%–95.1% with vaccine strain CV777. The partial S gene deduced amino acid sequences were compared and also showed a high degree of homology (98.0%–100.0%); they had 85.3%–98.7% identity with all reference strains listed in Technical Appendix Table 2, 98.0%–98.7% with Thailand strains, and 93.3%–94.7% with vaccine strain CV777 (data not shown). Phylogenetic analysis indicated that the PEDV in the China outbreak was different from foreign and other domestic strains on the basis of the reported partial S gene sequences. All new strains were clustered in the same branch, close to the cluster of Thailand strains, and far from the cluster of vaccine strain CV777 (Figure). Figure Phylogenetic tree constructed by using the neighbor-joining method based on the 9 porcine epidemic diarrhea virus (PEDV) sequences identified in a study of porcine epidemic diarrhea in China. Partially amplified spike genes of the PEDV isolates plus 18 PEDV sequences downloaded from GenBank were compared. Sequences included in each cluster are listed in Technical Appendix Table 3. Strains from Thailand and China and the CV777 vaccine strain are indicated. Scale bar indicates nucleotide substitutions per site. In the China outbreak, PEDV caused severe diarrheal disease in piglets; heavy economic losses in many provinces resulted, despite use of commercial vaccines (inactivated transmissible gastroenteritis [TGEV H] and porcine epidemic diarrhea [CV777]). To determine why the vaccines showed poor efficacy, we investigated evolution of the virus. Comparison of amino acid sequences from isolates from the outbreak and from the CV777 vaccine strain showed 9 amino acid mutations of fragments containing major hydrophilic regions: 16 (L→H), 18 (S→G), 22 (V→I), 44 (T→S), 89 (G→S), 100 (A→E), 107 (L→F), 130 (I→V) and 160 (I→F) (Technical Appendix Figure, panel A). Three of these 9 mutations were at positions 16, 18, and 22 in the isolates from China; they influenced the hydrophobicity of the S protein as compared with that for CV777 (Technical Appendix Figure, panel B). Phylogenic analysis showed that strain CV777 did not cluster with current common strains and showed considerable genetic distance from them. Isolates in the outbreak in China had only a minor nucleotide sequence variation from the Thailand isolates, indicating that the virus has a high genetic relatedness to the Southeast Asia strain. However, previous studies showed that isolates from Europe, South Korea, and China were serologically identical to the prototype CV777 strain ( 1 , 4 ). To our knowledge, fecal–oral transmission is probably the main or only route of PEDV transmission ( 5 – 7 ). In our study, if a fecal sample from a sick piglet was found to be positive for PEDV, we also collected and studied milk from its mother. These results showed that PEDV was present in sow milk (Technical Appendix Table 3), but the detection rate was lower for these samples (40.8%) than for the fecal samples (82.0%). On the basis of these results, we hypothesize that sow milk could represent a possible (and potentially major) route for the vertical transmission of PEDV from sow to suckling piglet. This hypothesis could be indirectly verified by our field observation that piglet death rates decreased as a result of fostering (data not shown). Our findings show that PEDV was identified not only in fecal samples from sick piglets, as expected, but also in the milk of the sow, which suggests vertical transmission of the virus. Supplementary Material Technical Appendix Current farms status in this study, China.

                Author and article information

                Journal
                Pathogens
                Pathogens
                pathogens
                Pathogens
                MDPI
                2076-0817
                21 March 2020
                March 2020
                : 9
                : 3
                : 233
                Affiliations
                [1 ]Veterinary Diagnostic and Production Animal Medicine, College of Veterinary Medicine, Iowa State University, Ames, IA 50010, USA; kkb@ 123456iastate.edu (K.K.-B.); juanmora@ 123456iastate.edu (J.C.M.-D.); jnb@ 123456iastate.edu (J.B.-K.); rmain@ 123456iastate.edu (R.M.)
                [2 ]Perkin Elmer, Waltham, MA 02451, USA; Philippe.Roby@ 123456perkinelmer.com (P.R.); Roger.Bosse@ 123456perkinelmer.com (R.B.)
                Author notes
                [* ]Correspondence: luisggl@ 123456iastate.edu ; Tel.: +1-515-294-7025
                Author information
                https://orcid.org/0000-0002-0725-122X
                Article
                pathogens-09-00233
                10.3390/pathogens9030233
                7157568
                32245150
                30d727af-7dc2-406d-934e-d0071ff1a2a7
                © 2020 by the authors.

                Licensee MDPI, Basel, Switzerland. This article is an open access article distributed under the terms and conditions of the Creative Commons Attribution (CC BY) license ( http://creativecommons.org/licenses/by/4.0/).

                History
                : 26 February 2020
                : 19 March 2020
                Categories
                Article

                porcine epidemic diarrhea virus,humoral immune response,serum igg,serum iga,alphalisa

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