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Identification of a novel cosavirus species in faeces of children and its relationship with acute gastroenteritis in China
Accepted Manuscript Identification of a novel cosavirus species in feces of children and its relationship with acute gastroenteritis in China Jie-mei Yu, Yuan-yun Ao, Li-li Li, Zhao-jun Duan PII:
S1198-743X(17)30110-6
DOI:
10.1016/j.cmi.2017.02.018
Reference:
CMI 866
To appear in:
Clinical Microbiology and Infection
Received Date: 1 July 2016 Revised Date:
8 February 2017
Accepted Date: 14 February 2017
Please cite this article as: Yu J-m, Ao Y-y, Li L-l, Duan Z-j, Identification of a novel cosavirus species in feces of children and its relationship with acute gastroenteritis in China, Clinical Microbiology and Infection (2017), doi: 10.1016/j.cmi.2017.02.018. This is a PDF file of an unedited manuscript that has been accepted for publication. As a service to our customers we are providing this early version of the manuscript. The manuscript will undergo copyediting, typesetting, and review of the resulting proof before it is published in its final form. Please note that during the production process errors may be discovered which could affect the content, and all legal disclaimers that apply to the journal pertain.
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Identification of a novel cosavirus species in feces of children and its relationship with
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acute gastroenteritis in China ⊥
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Jie-mei Yu , Yuan-yun Ao , Li-li Li, Zhao-jun Duan*
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Institute for Viral Diseases Control and Prevention, China CDC, Beijing 100052, China
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*Corresponding author: Zhao-jun Duan E-mail: [email protected]
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Telephone number: 86-10-63552910
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Fax number: 86-10-63557757
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These two authors contributed equally to the manuscript.
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Key words: novel Cosavirus; diarrhea; children; case-control study
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Running title:
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Association of a novel cosavirus with diarrhea
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ACCEPTED MANUSCRIPT Abstract
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Objectives: To assess the prevalence of human cosavirus (HCosV) in China and to
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determine the association of a novel HCosV (Cosa-CHN) with acute gastroenteritis (AGE) .
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Methods: A case-control study with 461 paired stool samples from diarrhea and healthy
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children was conducted. Real-time PCR and nested PCR were used to detect the HCosVs.
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Rapid-amplification of cDNA ends was employed to obtain the ends of the Cosa-CHN.
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Results: Known HCosVs were detected in two control samples, while Cosa-CHN was
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detected in eight (1.7%) and six (1.3%) of the case and control samples, respectively. The
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complete genome of Cosa-CHN comprises 7213 bp. The P1 and P2 regions of the
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Cosa-CHN were closely related to those of HCosV B, while the P3 region was most similar
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to that of HCosV D, albeit with low amino acid (aa) identities (66% and 67%, respectively).
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Phylogenetic analyses of the polyprotein and partial VP3/VP1 regions indicated that
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Cosa-CHN could be classified as a novel species (tentatively named HCosV G) in
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cosavirus. There was no significant difference in detection rate (p = 0.59) or mean viral
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load (p = 0.43) of Cosa-CHN between the cases and controls. Statistical analysis revealed
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no association between Cosa-CHN and AGE (p = 0.76), and the virus did not exacerbate
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clinical symptoms.
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Conclusions: A low prevalence of HCosV was detected, but a novel cosavirus species was
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found in children with and without gastroenteritis in this study, and the evidence did not
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support a causative role for the novel virus in pediatric AGE.
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Introduction
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Picornaviridae is a large family of viruses with a naked capsid surrounding a core of
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single-stranded, positive-sense genomic RNA encoding a single polyprotein. With the
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advent of high-throughput sequencing, an increasing number of novel picornaviruses have
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been described. As of July 2013, the family Picornaviridae comprised 26 genera
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(http://www.ictvonline.org/virusTaxonomy.asp), and included several leading pathogens
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that affect human and animal health; e.g., polioviruses and hand-foot-and-mouth-disease
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related enteroviruses.
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Human cosavirus (HCosV) is a novel virus that was first detected in fecal samples of
ACCEPTED MANUSCRIPT both healthy children and those with nonpolio acute flaccid paralysis in Pakistan in 2008
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[1]. Subsequently, the virus was found in feces from diverse populations and in sewage
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water worldwide [2,3,4,5,6,7,8]. The closest relatives of HCosV among the picornaviruses
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are cardioviruses and senecavirus. The International Committee on the Taxonomy of
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Viruses (ICTV) states that the genus cosavirus comprises a single type species (species A)
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(http://www.ictvonline.org/virusTaxonomy.asp). However, five additional species (B to F)
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of at least 30 genotypes have been reported [1,2,8,9].
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A recent study from Japan suggested HCosV to be a causal pathogen in pediatric
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patients because of the absence of other common diarrhea-causing viruses [8]. However,
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according to a previous study, the prevalence of HCosV varies geographically from 0.1% to
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48%. Moreover, because of frequent viral co-infection and low HCosV loads, the human
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pathogenicity of cosavirus is controversial [5]. Furthermore, the marked genetic diversity of
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HCosV complicates disease-association studies, as different viral types are likely associated
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with different symptoms. Here, we conducted a strict 1:1 paired case-control study to
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investigate the prevalence of cosavirus in Chinese children and its relationship with acute
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gastroenteritis (AGE). A novel human cosavirus species (Cosa-CHN) was found in this
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study to be the most prevalent cosavirus.
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Materials and Methods
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Samples
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Two hundred thirty-nine and two hundred twenty-two pairs of fecal samples from children
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less than 5 years of age were collected in Lulong, Hebei Province, and Liuyang, Hunan
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Province, respectively, from 2011 to 2013, as described in our recent study [10]. Briefly,
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cases were individuals diagnosed by a pediatrician with diarrhea without other diagnosed
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illness, such as pneumonia. Control subjects were healthy children who did not have
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diarrhea, fever, vomiting, or a respiratory illness during the previous 1 week. Samples from
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the controls were collected by village doctor from the children's home, and the maximum
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time interval between matched case and control sampling was 14 days. The healthy and
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diarrhea subjects were paired according to age (age groups: 0-5, 6-11, 12-23, 24-35, 36-47
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and 48-59 months), sex, and area.
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Only one specimen was obtained per patient. All stool specimens were collected
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was obtained from the parents of all children who provided specimens. The study protocol
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was approved by a meeting of the Ethics Committee of the National Institute for Viral
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Disease Control and Prevention, China Center for Disease Control, according to Chinese
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ethics laws and regulations.
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Detection of Common Diarrhea-Related Viruses
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Viral nucleotides were extracted from 10% fecal suspensions in phosphate-buffered saline
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using the QIAamp Viral RNA MiniKit (Qiagen), and first-strand cDNAs were synthesized
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using the Superscript II reverse transcriptase (Invitrogen) with random primers. All
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specimens were tested for rotavirus (RV), human calicivirus (HucV) (norovirus and
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sapovirus), astrovirus (AstV), and adenovirus (AdV) by real-time PCR using primers,
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probes, and reaction conditions reported previously [11,12,13,14]. The positivity rates of
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RV, HuCV, AdV, and AstV in the case and control groups were calculated as described in
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our previous study [10].
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Human Cosavirus Detection
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HCosV was detected by real-time PCR using primers and conditions described previously
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[5]. Positive samples were confirmed and genotyped by nested PCR amplification of a
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904-bp fragment of the viral capsid gene using primers described elsewhere [9]. The
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products were purified using a QIAquick PCR Purification Kit (Qiagen) and sequenced.
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One sequence with low homology (aa identity <65%) to previously reported HCosV was
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detected. The complete genome of this novel virus was amplified. The three sequences
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were submitted to GenBank under accession numbers KP213320–KP213322.
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Complete Genomic Amplification
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To determine the complete genome sequence of Cosa-CHN, we designed primers based on
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the sequence amplified by nested PCR. Further synthesis was based on the newly amplified
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sequences. PCR amplifications were performed using a Genome Walking Kit (TaKaRa,
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Japan) and the extreme 5′ and 3′ ends of the genome were determined using a SMART
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RACE cDNA Amplification Kit (Clontech) following the manufacturer’s instructions.
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Sequences were assembled and edited manually to produce the final sequence of the viral
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genome. Overlapping long fragments (1228–2989 bp) were amplified for final confirmation
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using ExTaq polymerase.
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Novel Cosavirus (Cosa-CHN) Detection
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Samples were screened for the novel cosavirus (Cosa-CHN) by nested PCR using upstream
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primers targeted to VP3 and downstream primers targeted to VP1. Primers for the first PCR
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round were CosF1 and CosR1 (supplemental table), and amplification was performed under
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standard PCR conditions with an initial five cycles of annealing at 56°C followed by 15
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cycles of annealing at 53°C. The second PCR round used the primers CosF2 and CosR2
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(supplemental table) under standard PCR conditions with an initial five cycles of annealing
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at 56°C followed by 35 cycles of annealing at 53°C. Positive and negative controls were
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included.
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Cosa-CHN viral loads in positive samples were quantified by real-time PCR. A
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forward primer (CosutrF), a reverse primer (CosutrR), and a probe (CosutrProbe) were
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designed to target the 5′ untranslated region (UTR) of the virus (supplemental table). The in
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vitro transcribed viral RNA was used as positive control. The reaction conditions were as
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follows: 50°C for 30 min, 95°C for 15 min, followed by 45 cycles of 95°C for 15 s and
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60°C for 1 min. After completion of amplification, fluorescence intensity was measured.
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Sequence and Phylogenetic Analysis
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PCR products were purified using a QIAquick PCR Purification Kit (Qiagen) and then sent
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for sequencing. Sequences were determined and analyzed using the DNAStar software
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package. The SimPlot software (version 3.5.1) was used to align and compare sequences to
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identify potential recombination of Cosa-CHN with other known cosavirus species.
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Phylogenetic analysis was performed using nucleotide sequences by the neighbor-joining
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method and subsequently subjected to bootstrap analysis with 1000 replicates to determine
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the reliability values at each internal node. Trees were produced using the MEGA software
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(version 5).
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Statistical Analysis
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The statistical significance of differences in mean viral loads between the groups was
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assessed using Student’s t-test, and that of differences in frequency among areas was
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evaluated using the Fisher’s exact test. Differences in clinical symptoms between groups
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were assessed by multiple factor logistic regression. P<0.05 was considered statistically
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significant. All statistical analyses were performed using SPSS 16.0.
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Results
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Detection of HCosV
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The results of screening real-time PCR showed that of the 461 pairs of samples, 3 (sample
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IDs: 67c, 87c, and 144) were positive for cosavirus, with viral loads of 1.07 × 104 copies/ml,
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4.94 × 102 copies/ml, and 2.98 × 104 copies/ml, respectively. Nested PCR and sequencing
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analysis suggested that samples 67c and 87c had the highest similarity to HCosV A17
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(Country: Nigeria), with 94 and 95% aa identities, respectively, while sample 144 was most
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similar to HCosV B1(Country: Pakistan), albeit with only 63% aa identity.
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Complete Genome of Cosa-CHN
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The low aa identity to HCosV B1 suggested the presence of a novel cosavirus (named
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Cosa-CHN), the complete genome of which was sequenced. A total of nine fragments were
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amplified to determine the complete genome sequence (Figure 1). The full-length genome
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sequence was deposited in GenBank under the accession number KM516909
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(NC_025961.1). The identified Cosa-CHN genome comprised 7213 bp (excluding the
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polyadenylated tract), with a 759-bp 5′ UTR, an open reading frame of 6360 nt (encoding a
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potential polyprotein precursor of 2120 aa), followed by a 94-bp 3′ UTR and poly(A) tail.
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The base usage of the Cosa-CHN genome was 28.9% A, 21.5% C, 20.7% G, and 28.9% U,
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with a relatively low G+C content (42.2%), which is similar to previously reported HCosVs
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[1]. A methionine start codon at nucleotide position 760 was found in the standard Kozak
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context (RNNAUGG was AAUAUGG). A hypothetical cleavage map of the Cosa-CHN
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polyprotein was derived from alignments with other HCosVs (Figure 1).
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The sequence of the P1 and P2 regions of Cosa-CHN exhibited 66% aa identity with
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those of its closest relative, HCosV B1. However, the P3 region of Cosa-CHN was most
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similar to that of HCosV D, with 67% aa identity. The 2C and 3CD regions of Cosa-CHN
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showed 70 and 67% aa identities with those of HCosV B1 and D, respectively. The ICTV
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states that enteroviruses in the picornaviridae sharing 70% aa identity in P1 and >70% aa
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identity in the 2C and 3CD regions belong to the same species [15]. Therefore, Cosa-CHN
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is proposed as a novel cosavirus species.
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Screening and Viral Loads of Cosa-CHN
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By using the Cosa-CHN-specific detection assay, a total of 461 pairs of samples were
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screened using nested PCR of the VP3/VP1 region of Cosa-CHN, together with sample ID
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144, and six (1.3%) controls (sample 67c and 87c that positive for HCosV were not positive
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for Cosa-CHN) and seven (1.7%) cases were positive for Cosa-CHN. These 13 sequences
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were submitted to GenBank under accession numbers KP213307–KP213319. All 14
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sequences of Cosa-CHN (including that of ID 144) with 256 bp spanning the VP3/VP1
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region showed 99% nt identities. The viruses were detected year-round; their distribution
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did not differ seasonally. Of the 14 Cosa-CHN-positive subjects, 3 were from Liuyang
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(South China) and 11 were from Lulong (North China). The age range of
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Cosa-CHN–positive case subjects was 3–15 months (median = 6.5 months), while that of
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Cosa-CHN–positive control subjects was 10–36 months (median = 11.5 months). A χ2- test
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revealed that detection rates differed significantly according to area (p = 0.005), but not
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between the case and control groups (p = 0.59). The detection rate of Cosa-CHN in
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Liuyang (southern China) and Lulong (northern China) Provinces differed significantly
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(4.5% vs. 1.7%).
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The mean viral load of the case group was 1.75 × 103 copies/mL (3.48 × 101–1.07 ×
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104 copies/mL) vs. 3.36 × 102 copies/mL (1.04 × 102–1.09 × 103 copies/mL) in the control
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group (Table); a log-normal t-test revealed no difference between the cases and controls (p
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= 0.43).
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Recombination and Phylogenetic Analysis of Cosa-CHN
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Recombination analysis showed no putative inter-species recombination in Cosa-CHN. A
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phylogenetic analysis using the nucleotide sequences of the VP3–VP1 region (Figure 2a)
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and complete polyprotein amino acid sequences (Figure 2b) of Cosa-CHN and other known
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HCosVs and other representative picornaviruses using the neighbor-joining method and
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1,000 bootstrap replications suggested that Cosa-CHN forms a distinct lineage. The two
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phylogenetic trees also showed that Cosa-CHN is more closely related to HCosV B than to
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other previously reported HCosVs.
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Association between Cosa-CHN and AGE Of the eight Cosa-CHN-positive children in the case group, five were co-infected with
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diarrhea-related viruses (Table). Infection with Cosa-CHN did not exacerbate the clinical
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symptoms (i.e., proportion of fever, frequency of diarrhea, and duration of diarrhea) of
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these children (data not shown).
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Discussion
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Cosavirus is a newly established genus in the family Picornaviridae that comprises six
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genetically distinct species (A–F) [9]. Following its discovery, HCosVs were reported in
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diverse sample types, including human feces, sewage, and porcine feces, in several
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countries, such as China, Italy, Thailand, Bolivia, Japan, Tunisia, and Brazil
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[1,2,3,4,5,6,8,16,17,18,19,20]. However, the prevalence ranges from 0 to 71% depending
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on the area and population. In this study, we used the real-time PCR method reported in a
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Brazilian study [5]. Only three samples from healthy children were positive for HCosVs,
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one of which exhibited the highest similarity to HCosV B, albeit with a low sequence
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identity. The complete genome of this virus was amplified, and the sequence suggested it to
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be a novel species of cosavirus, tentatively named Cosa-CHN.
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The genome structure of Cosa-CHN was similar to that of other HCosVs, comprising 5' UTR–structural proteins (VP4, VP2, VP3, and VP1)–non-structural proteins (2A–2C and
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3A–3D)–3' UTR–poly (A) tail. The length of 5'UTR of Cosa-CHN (759bp) is similar to
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that of those previously published HCosVs (HCosV B,FJ438907, 749bp; HCosV D,
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FJ438908, 747bp), it is estimated that the complete sequence of 5'UTR of Cosa-CHN. The
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cleavage sites in structural proteins, but not non-structural proteins, differ markedly among
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HCosVs; however, the putative cleavage sites for Cosa-CHN and HCosV-B were identical,
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with the exception of one difference in VP4 and VP1 (A/D and A/S, respectively). The
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common motifs in the non-structural proteins of picornaviruses, such as the NTPase and
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helicase motifs, were also found in Cosa-CHN. However, unlike many picornaviral
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genomes, which contain a leader (L) protein, the genome of HCosV has no L protein at the
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5′ end, similar to hepataviruses, enteroviruses, and hepatoviruses [21]. Moreover,
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Cosa-CHN lacked the VP1 RGD motif, which is present in other HCosVs.
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Sequence analysis revealed that the P1 and P2 regions of Cosa-CHN showed the highest similarity to those of HCosV-B, while the P3 region was most similar to that of
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HCosV-D; however, all aa identity values were low (<70%). Although picornavirus
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recombination is frequently observed within, but not between, viral species, with the
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exception of exchange of the regulatory 5′ UTR region [22,23], the recombinant HCosV
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D/E strain found in a previous study that exhibited recombination at the P1/P2 junction was
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designated a single species [9]. Recombination analysis showed no recombination event in
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Cosa-CHN. Phylogenetic analyses of the polyprotein and VP3/VP1 indicated that this virus
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forms a separate branch to previous HCosVs, suggesting that Cosa-CHN represents a novel
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species. The marked genetic diversity of HCosVs suggests a wide range of effects on the
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host, as is the case for the similarly diverse enteroviruses.
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Primers for screening HCosV matched HCosV A–F well, but Cosa-CHN less well, as three nucleotides differed in each real time PCR primer (mismatched in position 12/13/15
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of the positive primer and in position 5/7/8 of the negative primer ). Therefore, it was
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unsurprising that Cosa-CHN could be amplified using these primers. However, it may be
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that low Cosa-CHN viral load infections were hard to detect with initial screening primers
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although this seem unlikely as ID 144 had the lowest viral load. In this study, the detection
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rate of known HCosVs was 0.2% (2/922), markedly lower than reported in Shanghai, China
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(3.2% in children with diarrhea and 1.6% in healthy children) [4], but similar to rates
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reported previously in the UK, Thailand, Japan, and Italy (0.1–0.5%) [6,8,20,22]. To
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evaluate the prevalence of Cosa-CHN, we designed specific primers; the Cosa-CHN
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detection rates were 1.3 and 1.7% in the case and control groups, respectively. Furthermore,
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the detection rate of Cosa-CHN in Liuyang (southern China) and Lulong (northern China)
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Provinces differed significantly (4.5% vs. 1.7%). Therefore, the prevalence of Cosa-CHN
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differed according to geographical area. Furthermore, Cosa-CHN-positive samples from
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both areas were collected year-round, suggestive of no seasonal difference in distribution
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(data not shown). This is unlike other enteric viruses, such as enterovirus, the prevalence of
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most of which varies seasonally but not geographically [24].
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The prevalence of Cosa-CHN, particularly in other countries, should be investigated further. The incidence of HCosV in raw sewage and river water in Japan (71 and 29%,
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as sewage is collection of samples from multiple persons. HCosV was also detected in pig
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stools in Bolivia, Thailand, and Japan (51.8, 55.4, and 18.9%, respectively). These data
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suggest that the distribution of cosavirus species may differ among environmental sources,
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populations and geographical areas. Interestingly, when using the specific primers (both
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nested PCR primers and real time PCR primers) used in this study to screen the
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Cosa-CHN-postive samples about three years later, it showed that all the samples were
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negative for Cosa-CHN. This phenomenon should be caused by the degradation of the virus
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in the sample, which indicates that this virus is not stable and the future study for this virus
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should be done using the fresh specimens.
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The pathogenicity of HCosV in humans remains unclear, as the wide genetic diversity
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and ubiquity of the virus complicates disease-association studies. Nevertheless, HCosV has
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been detected in subjects with diarrhea; e.g., two previous studies from Japan demonstrated
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that HCosV might cause diarrhea in pediatric patients [8,25]. In this study, two samples
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from healthy children were positive for known HCosVs, so we evaluated the relationship
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between Cosa-CHN and AGE in children. There was no difference in the detection rate and
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mean viral load of Cosa-CHN between the case and control subjects. However, coinfection
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with other diarrhea-related viruses was frequent in the Cosa-CHN-positive samples from
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the case group (5/8). Further statistical analysis indicated that Cosa-CHN coinfection did
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not exacerbate the clinical symptoms of gastroenteritis. Taken together, these findings
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suggest that Cosa-CHN does not play a role in gastroenteritis. However, it should be noted
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that the viral loads were relatively low in this study. A previous study reported that
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norovirus viral loads lower than a threshold level, it should be regarded as negative; in
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other word, though the virus was detected, it was not a causal factor in the disease [26].
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This might also be the case for Cosa-CHN infection, so the possibility that a high load of
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Cosa-CHN may cause diarrhea cannot be ruled out. Moreover, specific cosavirus genotypes
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may yet be shown to be associated with specific diseases as is the case for enteroviruses.
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Further studies involving virus stability, virus isolation, animal experiments, serology and
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molecular epidemiology should be performed to evaluate the pathogenicity of different
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cosavirus species and genotypes.
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Funding information
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This work was supported by the National Natural Science Foundation of China (Grant No.
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81290345).
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Competing interest
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All authors declare no conflict of interest.
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Author contribution
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ZJD and JMY designed the experiments; JMY, YYA and LLL performed the experiments;
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JMY and YYA analyzed the results; JMY wrote the draft manuscript. ZJD revised the
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manuscript. All the authors reviewed the manuscript.
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11. Chan MC, Sung JJ, Lam RK, Chan PK, Lai RW, et al. (2006) Sapovirus detection by quantitative
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Figure legends
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Figure 1. (a) genome organization of Cosa-CHN; (b) whole virus sequencing approach; and
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(c) protein cleavage map. Nine fragments were used to produce the final genome sequence.
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The potential cleavage sites of Cosa-CHN are similar to those of HCosV B. The location of
real-time RT-PCR in clinical stool specimens. J Virol Methods 134: 146-153. 12. Kageyama T, Kojima S, Shinohara M, Uchida K, Fukushi S, et al. (2003) Broadly reactive and highly sensitive assay for Norwalk-like viruses based on real-time quantitative reverse transcription-PCR. J Clin Microbiol 41: 1548-1557. 13. Pang XL, Lee B, Boroumand N, Leblanc B, Preiksaitis JK, et al. (2004) Increased detection of rotavirus using a real time reverse transcription-polymerase chain reaction (RT-PCR) assay in stool specimens
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from children with diarrhea. J Med Virol 72: 496-501.
14. Wolffs PF, Bruggeman CA, van Well GT, van Loo IH. (2011) Replacing traditional diagnostics of fecal viral pathogens by a comprehensive panel of real-time PCRs. J Clin Microbiol 49: 1926-1931. 15. Fauquet. C, Mayo. M, J. M, U. D, LA. B (2005) Virus taxonomy: Eighth report of the International Committee on Taxonomy of Viruses. San Diego, CA: Elsevier Academic Press.
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16. Okitsu S, Khamrin P, Hanaoka N, Thongprachum A, Takanashi S, et al. (2016) Cosavirus (family Picornaviridae) in pigs in Thailand and Japan. Arch Virol 161: 159-163.
17. Khamrin P, Chaimongkol N, Malasao R, Suantai B, Saikhruang W, et al. (2012) Detection and molecular characterization of cosavirus in adults with diarrhea, Thailand. Virus Genes 44: 244-246.
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18. Nix WA, Khetsuriani N, Penaranda S, Maher K, Venczel L, et al. (2013) Diversity of picornaviruses in rural Bolivia. J Gen Virol 94: 2017-2028.
19. Rezig D, Ben Farhat E, Touzi H, Meddeb Z, Ben Salah A, et al. (2015) Prevalence of human cosaviruses in Tunisia, North Africa. J Med Virol 87: 940-943.
20. Kitajima M, Rachmadi AT, Iker BC, Haramoto E, Pepper IL, et al. (2015) Occurrence and genetic diversity of human cosavirus in influent and effluent of wastewater treatment plants in Arizona, United States. Arch Virol 160: 1775-1779.
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21. Yamashita T, Sakae K, Tsuzuki H, Suzuki Y, Ishikawa N, et al. (1998) Complete nucleotide sequence and genetic organization of Aichi virus, a distinct member of the Picornaviridae associated with acute gastroenteritis in humans. J Virol 72: 8408-8412. 22. Santti J, Hyypia T, Kinnunen L, Salminen M (1999) Evidence of recombination among enteroviruses. J Virol 73: 8741-8749.
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23. Simmonds P, Welch J (2006) Frequency and dynamics of recombination within different species of human enteroviruses. J Virol 80: 483-493. 24. Xing W, Liao Q, Viboud C, Zhang J, Sun J, et al. (2014) Hand, foot, and mouth disease in China, 2008-12:
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an epidemiological study. Lancet Infect Dis 14: 308-318. 25. Okitsu S, Khamrin P, Thongprachum A, Nishimura S, Kalesaran AF, et al. (2014) Detection and molecular characterization of human cosavirus in a pediatric patient with acute gastroenteritis, Japan. Infect Genet Evol 28: 125-129.
26. Phillips G, Lopman B, Tam CC, Iturriza-Gomara M, Brown D, et al. (2009) Diagnosing norovirus-associated infectious intestinal disease using viral load. BMC Infect Dis 9: 63.
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the initial PCR for HCosV and Cosa-CHN specific RT-nPCR amplicon products were in
376
red and marked as "VP1" and "VP3/VP1" ,respectively.
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Figure 2. Phylogenetic analysis of Cosa-CHN sequences: (a) polyprotein amino acid
379
sequences; (b) partial VP3/VP1 nucleotide sequences. The tree was constructed using the
380
neighbor-joining method b ny MEGA ver. 5 with 1,000 bootstrap replicates. Sequences
381
from this study are indicated by "•". Cosa-CHN formed a lineage distinct from other known
382
HCosV.
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ACCEPTED MANUSCRIPT Table 1. Clinical characteristics, viral loads, and related information of eight children in the case group positive for Cosa-CHN. Duration of Patient ID
diarrhea,
Age,
Frequency of
Viral load,
diarrhea, per
copies
Sex
Area
days
Month
Coinfection
Fever
day
Vomiting
(copies/ml)
144
F
Hunan
7
8
HuCV
+
4
-
3.48×101
038
F
Hebei
3
8
-
+
061
F
Hunan
2
6
RV, AdV
+
070
M
Hunan
2
7
AstV
-
102
F
Hunan
1
3
-
N
052
M
Hunan
3
6
-
113
M
Hebei
2
15
RV
073
F
Hebei
15
4
RV
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No.
-
8.36×101
2
+
1.05×102
6
-
3.46×102
2
-
3.65×102
+
4
-
5.02×102
-
7
-
1.90×103
-
6
+
1.07×104
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Note: Duration of diarrhea indicates the time from the date of admission to the date of
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discharge from hospital. M, male; F, female; N, no data; +, present; -, absent.
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S1198-743X(17)30110-6
DOI:
10.1016/j.cmi.2017.02.018
Reference:
CMI 866
To appear in:
Clinical Microbiology and Infection
Received Date: 1 July 2016 Revised Date:
8 February 2017
Accepted Date: 14 February 2017
Please cite this article as: Yu J-m, Ao Y-y, Li L-l, Duan Z-j, Identification of a novel cosavirus species in feces of children and its relationship with acute gastroenteritis in China, Clinical Microbiology and Infection (2017), doi: 10.1016/j.cmi.2017.02.018. This is a PDF file of an unedited manuscript that has been accepted for publication. As a service to our customers we are providing this early version of the manuscript. The manuscript will undergo copyediting, typesetting, and review of the resulting proof before it is published in its final form. Please note that during the production process errors may be discovered which could affect the content, and all legal disclaimers that apply to the journal pertain.
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Identification of a novel cosavirus species in feces of children and its relationship with
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acute gastroenteritis in China ⊥
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⊥
Jie-mei Yu , Yuan-yun Ao , Li-li Li, Zhao-jun Duan*
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Institute for Viral Diseases Control and Prevention, China CDC, Beijing 100052, China
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*Corresponding author: Zhao-jun Duan E-mail: [email protected]
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Telephone number: 86-10-63552910
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Fax number: 86-10-63557757
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⊥
These two authors contributed equally to the manuscript.
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Key words: novel Cosavirus; diarrhea; children; case-control study
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Running title:
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Association of a novel cosavirus with diarrhea
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ACCEPTED MANUSCRIPT Abstract
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Objectives: To assess the prevalence of human cosavirus (HCosV) in China and to
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determine the association of a novel HCosV (Cosa-CHN) with acute gastroenteritis (AGE) .
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Methods: A case-control study with 461 paired stool samples from diarrhea and healthy
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children was conducted. Real-time PCR and nested PCR were used to detect the HCosVs.
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Rapid-amplification of cDNA ends was employed to obtain the ends of the Cosa-CHN.
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Results: Known HCosVs were detected in two control samples, while Cosa-CHN was
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detected in eight (1.7%) and six (1.3%) of the case and control samples, respectively. The
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complete genome of Cosa-CHN comprises 7213 bp. The P1 and P2 regions of the
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Cosa-CHN were closely related to those of HCosV B, while the P3 region was most similar
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to that of HCosV D, albeit with low amino acid (aa) identities (66% and 67%, respectively).
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Phylogenetic analyses of the polyprotein and partial VP3/VP1 regions indicated that
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Cosa-CHN could be classified as a novel species (tentatively named HCosV G) in
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cosavirus. There was no significant difference in detection rate (p = 0.59) or mean viral
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load (p = 0.43) of Cosa-CHN between the cases and controls. Statistical analysis revealed
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no association between Cosa-CHN and AGE (p = 0.76), and the virus did not exacerbate
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clinical symptoms.
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Conclusions: A low prevalence of HCosV was detected, but a novel cosavirus species was
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found in children with and without gastroenteritis in this study, and the evidence did not
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support a causative role for the novel virus in pediatric AGE.
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Introduction
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Picornaviridae is a large family of viruses with a naked capsid surrounding a core of
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single-stranded, positive-sense genomic RNA encoding a single polyprotein. With the
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advent of high-throughput sequencing, an increasing number of novel picornaviruses have
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been described. As of July 2013, the family Picornaviridae comprised 26 genera
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(http://www.ictvonline.org/virusTaxonomy.asp), and included several leading pathogens
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that affect human and animal health; e.g., polioviruses and hand-foot-and-mouth-disease
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related enteroviruses.
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Human cosavirus (HCosV) is a novel virus that was first detected in fecal samples of
ACCEPTED MANUSCRIPT both healthy children and those with nonpolio acute flaccid paralysis in Pakistan in 2008
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[1]. Subsequently, the virus was found in feces from diverse populations and in sewage
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water worldwide [2,3,4,5,6,7,8]. The closest relatives of HCosV among the picornaviruses
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are cardioviruses and senecavirus. The International Committee on the Taxonomy of
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Viruses (ICTV) states that the genus cosavirus comprises a single type species (species A)
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(http://www.ictvonline.org/virusTaxonomy.asp). However, five additional species (B to F)
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of at least 30 genotypes have been reported [1,2,8,9].
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A recent study from Japan suggested HCosV to be a causal pathogen in pediatric
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patients because of the absence of other common diarrhea-causing viruses [8]. However,
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according to a previous study, the prevalence of HCosV varies geographically from 0.1% to
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48%. Moreover, because of frequent viral co-infection and low HCosV loads, the human
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pathogenicity of cosavirus is controversial [5]. Furthermore, the marked genetic diversity of
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HCosV complicates disease-association studies, as different viral types are likely associated
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with different symptoms. Here, we conducted a strict 1:1 paired case-control study to
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investigate the prevalence of cosavirus in Chinese children and its relationship with acute
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gastroenteritis (AGE). A novel human cosavirus species (Cosa-CHN) was found in this
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study to be the most prevalent cosavirus.
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Materials and Methods
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Samples
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Two hundred thirty-nine and two hundred twenty-two pairs of fecal samples from children
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less than 5 years of age were collected in Lulong, Hebei Province, and Liuyang, Hunan
77
Province, respectively, from 2011 to 2013, as described in our recent study [10]. Briefly,
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cases were individuals diagnosed by a pediatrician with diarrhea without other diagnosed
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illness, such as pneumonia. Control subjects were healthy children who did not have
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diarrhea, fever, vomiting, or a respiratory illness during the previous 1 week. Samples from
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the controls were collected by village doctor from the children's home, and the maximum
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time interval between matched case and control sampling was 14 days. The healthy and
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diarrhea subjects were paired according to age (age groups: 0-5, 6-11, 12-23, 24-35, 36-47
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and 48-59 months), sex, and area.
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Only one specimen was obtained per patient. All stool specimens were collected
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was obtained from the parents of all children who provided specimens. The study protocol
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was approved by a meeting of the Ethics Committee of the National Institute for Viral
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Disease Control and Prevention, China Center for Disease Control, according to Chinese
90
ethics laws and regulations.
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Detection of Common Diarrhea-Related Viruses
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Viral nucleotides were extracted from 10% fecal suspensions in phosphate-buffered saline
93
using the QIAamp Viral RNA MiniKit (Qiagen), and first-strand cDNAs were synthesized
94
using the Superscript II reverse transcriptase (Invitrogen) with random primers. All
95
specimens were tested for rotavirus (RV), human calicivirus (HucV) (norovirus and
96
sapovirus), astrovirus (AstV), and adenovirus (AdV) by real-time PCR using primers,
97
probes, and reaction conditions reported previously [11,12,13,14]. The positivity rates of
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RV, HuCV, AdV, and AstV in the case and control groups were calculated as described in
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our previous study [10].
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Human Cosavirus Detection
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HCosV was detected by real-time PCR using primers and conditions described previously
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[5]. Positive samples were confirmed and genotyped by nested PCR amplification of a
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904-bp fragment of the viral capsid gene using primers described elsewhere [9]. The
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products were purified using a QIAquick PCR Purification Kit (Qiagen) and sequenced.
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One sequence with low homology (aa identity <65%) to previously reported HCosV was
106
detected. The complete genome of this novel virus was amplified. The three sequences
107
were submitted to GenBank under accession numbers KP213320–KP213322.
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Complete Genomic Amplification
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To determine the complete genome sequence of Cosa-CHN, we designed primers based on
110
the sequence amplified by nested PCR. Further synthesis was based on the newly amplified
111
sequences. PCR amplifications were performed using a Genome Walking Kit (TaKaRa,
112
Japan) and the extreme 5′ and 3′ ends of the genome were determined using a SMART
113
RACE cDNA Amplification Kit (Clontech) following the manufacturer’s instructions.
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Sequences were assembled and edited manually to produce the final sequence of the viral
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genome. Overlapping long fragments (1228–2989 bp) were amplified for final confirmation
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using ExTaq polymerase.
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Novel Cosavirus (Cosa-CHN) Detection
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Samples were screened for the novel cosavirus (Cosa-CHN) by nested PCR using upstream
120
primers targeted to VP3 and downstream primers targeted to VP1. Primers for the first PCR
121
round were CosF1 and CosR1 (supplemental table), and amplification was performed under
122
standard PCR conditions with an initial five cycles of annealing at 56°C followed by 15
123
cycles of annealing at 53°C. The second PCR round used the primers CosF2 and CosR2
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(supplemental table) under standard PCR conditions with an initial five cycles of annealing
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at 56°C followed by 35 cycles of annealing at 53°C. Positive and negative controls were
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included.
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Cosa-CHN viral loads in positive samples were quantified by real-time PCR. A
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forward primer (CosutrF), a reverse primer (CosutrR), and a probe (CosutrProbe) were
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designed to target the 5′ untranslated region (UTR) of the virus (supplemental table). The in
130
vitro transcribed viral RNA was used as positive control. The reaction conditions were as
131
follows: 50°C for 30 min, 95°C for 15 min, followed by 45 cycles of 95°C for 15 s and
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60°C for 1 min. After completion of amplification, fluorescence intensity was measured.
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Sequence and Phylogenetic Analysis
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PCR products were purified using a QIAquick PCR Purification Kit (Qiagen) and then sent
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for sequencing. Sequences were determined and analyzed using the DNAStar software
136
package. The SimPlot software (version 3.5.1) was used to align and compare sequences to
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identify potential recombination of Cosa-CHN with other known cosavirus species.
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Phylogenetic analysis was performed using nucleotide sequences by the neighbor-joining
139
method and subsequently subjected to bootstrap analysis with 1000 replicates to determine
140
the reliability values at each internal node. Trees were produced using the MEGA software
141
(version 5).
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Statistical Analysis
143
The statistical significance of differences in mean viral loads between the groups was
144
assessed using Student’s t-test, and that of differences in frequency among areas was
145
evaluated using the Fisher’s exact test. Differences in clinical symptoms between groups
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were assessed by multiple factor logistic regression. P<0.05 was considered statistically
147
significant. All statistical analyses were performed using SPSS 16.0.
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Results
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Detection of HCosV
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The results of screening real-time PCR showed that of the 461 pairs of samples, 3 (sample
152
IDs: 67c, 87c, and 144) were positive for cosavirus, with viral loads of 1.07 × 104 copies/ml,
153
4.94 × 102 copies/ml, and 2.98 × 104 copies/ml, respectively. Nested PCR and sequencing
154
analysis suggested that samples 67c and 87c had the highest similarity to HCosV A17
155
(Country: Nigeria), with 94 and 95% aa identities, respectively, while sample 144 was most
156
similar to HCosV B1(Country: Pakistan), albeit with only 63% aa identity.
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Complete Genome of Cosa-CHN
158
The low aa identity to HCosV B1 suggested the presence of a novel cosavirus (named
159
Cosa-CHN), the complete genome of which was sequenced. A total of nine fragments were
160
amplified to determine the complete genome sequence (Figure 1). The full-length genome
161
sequence was deposited in GenBank under the accession number KM516909
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(NC_025961.1). The identified Cosa-CHN genome comprised 7213 bp (excluding the
163
polyadenylated tract), with a 759-bp 5′ UTR, an open reading frame of 6360 nt (encoding a
164
potential polyprotein precursor of 2120 aa), followed by a 94-bp 3′ UTR and poly(A) tail.
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The base usage of the Cosa-CHN genome was 28.9% A, 21.5% C, 20.7% G, and 28.9% U,
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with a relatively low G+C content (42.2%), which is similar to previously reported HCosVs
167
[1]. A methionine start codon at nucleotide position 760 was found in the standard Kozak
168
context (RNNAUGG was AAUAUGG). A hypothetical cleavage map of the Cosa-CHN
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polyprotein was derived from alignments with other HCosVs (Figure 1).
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The sequence of the P1 and P2 regions of Cosa-CHN exhibited 66% aa identity with
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those of its closest relative, HCosV B1. However, the P3 region of Cosa-CHN was most
172
similar to that of HCosV D, with 67% aa identity. The 2C and 3CD regions of Cosa-CHN
173
showed 70 and 67% aa identities with those of HCosV B1 and D, respectively. The ICTV
174
states that enteroviruses in the picornaviridae sharing 70% aa identity in P1 and >70% aa
175
identity in the 2C and 3CD regions belong to the same species [15]. Therefore, Cosa-CHN
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is proposed as a novel cosavirus species.
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Screening and Viral Loads of Cosa-CHN
179
By using the Cosa-CHN-specific detection assay, a total of 461 pairs of samples were
180
screened using nested PCR of the VP3/VP1 region of Cosa-CHN, together with sample ID
181
144, and six (1.3%) controls (sample 67c and 87c that positive for HCosV were not positive
182
for Cosa-CHN) and seven (1.7%) cases were positive for Cosa-CHN. These 13 sequences
183
were submitted to GenBank under accession numbers KP213307–KP213319. All 14
184
sequences of Cosa-CHN (including that of ID 144) with 256 bp spanning the VP3/VP1
185
region showed 99% nt identities. The viruses were detected year-round; their distribution
186
did not differ seasonally. Of the 14 Cosa-CHN-positive subjects, 3 were from Liuyang
187
(South China) and 11 were from Lulong (North China). The age range of
188
Cosa-CHN–positive case subjects was 3–15 months (median = 6.5 months), while that of
189
Cosa-CHN–positive control subjects was 10–36 months (median = 11.5 months). A χ2- test
190
revealed that detection rates differed significantly according to area (p = 0.005), but not
191
between the case and control groups (p = 0.59). The detection rate of Cosa-CHN in
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Liuyang (southern China) and Lulong (northern China) Provinces differed significantly
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(4.5% vs. 1.7%).
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The mean viral load of the case group was 1.75 × 103 copies/mL (3.48 × 101–1.07 ×
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104 copies/mL) vs. 3.36 × 102 copies/mL (1.04 × 102–1.09 × 103 copies/mL) in the control
196
group (Table); a log-normal t-test revealed no difference between the cases and controls (p
197
= 0.43).
198
Recombination and Phylogenetic Analysis of Cosa-CHN
199
Recombination analysis showed no putative inter-species recombination in Cosa-CHN. A
200
phylogenetic analysis using the nucleotide sequences of the VP3–VP1 region (Figure 2a)
201
and complete polyprotein amino acid sequences (Figure 2b) of Cosa-CHN and other known
202
HCosVs and other representative picornaviruses using the neighbor-joining method and
203
1,000 bootstrap replications suggested that Cosa-CHN forms a distinct lineage. The two
204
phylogenetic trees also showed that Cosa-CHN is more closely related to HCosV B than to
205
other previously reported HCosVs.
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Association between Cosa-CHN and AGE Of the eight Cosa-CHN-positive children in the case group, five were co-infected with
208
diarrhea-related viruses (Table). Infection with Cosa-CHN did not exacerbate the clinical
209
symptoms (i.e., proportion of fever, frequency of diarrhea, and duration of diarrhea) of
210
these children (data not shown).
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Discussion
213
Cosavirus is a newly established genus in the family Picornaviridae that comprises six
214
genetically distinct species (A–F) [9]. Following its discovery, HCosVs were reported in
215
diverse sample types, including human feces, sewage, and porcine feces, in several
216
countries, such as China, Italy, Thailand, Bolivia, Japan, Tunisia, and Brazil
217
[1,2,3,4,5,6,8,16,17,18,19,20]. However, the prevalence ranges from 0 to 71% depending
218
on the area and population. In this study, we used the real-time PCR method reported in a
219
Brazilian study [5]. Only three samples from healthy children were positive for HCosVs,
220
one of which exhibited the highest similarity to HCosV B, albeit with a low sequence
221
identity. The complete genome of this virus was amplified, and the sequence suggested it to
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be a novel species of cosavirus, tentatively named Cosa-CHN.
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The genome structure of Cosa-CHN was similar to that of other HCosVs, comprising 5' UTR–structural proteins (VP4, VP2, VP3, and VP1)–non-structural proteins (2A–2C and
225
3A–3D)–3' UTR–poly (A) tail. The length of 5'UTR of Cosa-CHN (759bp) is similar to
226
that of those previously published HCosVs (HCosV B,FJ438907, 749bp; HCosV D,
227
FJ438908, 747bp), it is estimated that the complete sequence of 5'UTR of Cosa-CHN. The
228
cleavage sites in structural proteins, but not non-structural proteins, differ markedly among
229
HCosVs; however, the putative cleavage sites for Cosa-CHN and HCosV-B were identical,
230
with the exception of one difference in VP4 and VP1 (A/D and A/S, respectively). The
231
common motifs in the non-structural proteins of picornaviruses, such as the NTPase and
232
helicase motifs, were also found in Cosa-CHN. However, unlike many picornaviral
233
genomes, which contain a leader (L) protein, the genome of HCosV has no L protein at the
234
5′ end, similar to hepataviruses, enteroviruses, and hepatoviruses [21]. Moreover,
235
Cosa-CHN lacked the VP1 RGD motif, which is present in other HCosVs.
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Sequence analysis revealed that the P1 and P2 regions of Cosa-CHN showed the highest similarity to those of HCosV-B, while the P3 region was most similar to that of
238
HCosV-D; however, all aa identity values were low (<70%). Although picornavirus
239
recombination is frequently observed within, but not between, viral species, with the
240
exception of exchange of the regulatory 5′ UTR region [22,23], the recombinant HCosV
241
D/E strain found in a previous study that exhibited recombination at the P1/P2 junction was
242
designated a single species [9]. Recombination analysis showed no recombination event in
243
Cosa-CHN. Phylogenetic analyses of the polyprotein and VP3/VP1 indicated that this virus
244
forms a separate branch to previous HCosVs, suggesting that Cosa-CHN represents a novel
245
species. The marked genetic diversity of HCosVs suggests a wide range of effects on the
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host, as is the case for the similarly diverse enteroviruses.
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Primers for screening HCosV matched HCosV A–F well, but Cosa-CHN less well, as three nucleotides differed in each real time PCR primer (mismatched in position 12/13/15
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of the positive primer and in position 5/7/8 of the negative primer ). Therefore, it was
250
unsurprising that Cosa-CHN could be amplified using these primers. However, it may be
251
that low Cosa-CHN viral load infections were hard to detect with initial screening primers
252
although this seem unlikely as ID 144 had the lowest viral load. In this study, the detection
253
rate of known HCosVs was 0.2% (2/922), markedly lower than reported in Shanghai, China
254
(3.2% in children with diarrhea and 1.6% in healthy children) [4], but similar to rates
255
reported previously in the UK, Thailand, Japan, and Italy (0.1–0.5%) [6,8,20,22]. To
256
evaluate the prevalence of Cosa-CHN, we designed specific primers; the Cosa-CHN
257
detection rates were 1.3 and 1.7% in the case and control groups, respectively. Furthermore,
258
the detection rate of Cosa-CHN in Liuyang (southern China) and Lulong (northern China)
259
Provinces differed significantly (4.5% vs. 1.7%). Therefore, the prevalence of Cosa-CHN
260
differed according to geographical area. Furthermore, Cosa-CHN-positive samples from
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both areas were collected year-round, suggestive of no seasonal difference in distribution
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(data not shown). This is unlike other enteric viruses, such as enterovirus, the prevalence of
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most of which varies seasonally but not geographically [24].
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The prevalence of Cosa-CHN, particularly in other countries, should be investigated further. The incidence of HCosV in raw sewage and river water in Japan (71 and 29%,
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267
as sewage is collection of samples from multiple persons. HCosV was also detected in pig
268
stools in Bolivia, Thailand, and Japan (51.8, 55.4, and 18.9%, respectively). These data
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suggest that the distribution of cosavirus species may differ among environmental sources,
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populations and geographical areas. Interestingly, when using the specific primers (both
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nested PCR primers and real time PCR primers) used in this study to screen the
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Cosa-CHN-postive samples about three years later, it showed that all the samples were
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negative for Cosa-CHN. This phenomenon should be caused by the degradation of the virus
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in the sample, which indicates that this virus is not stable and the future study for this virus
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should be done using the fresh specimens.
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The pathogenicity of HCosV in humans remains unclear, as the wide genetic diversity
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and ubiquity of the virus complicates disease-association studies. Nevertheless, HCosV has
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been detected in subjects with diarrhea; e.g., two previous studies from Japan demonstrated
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that HCosV might cause diarrhea in pediatric patients [8,25]. In this study, two samples
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from healthy children were positive for known HCosVs, so we evaluated the relationship
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between Cosa-CHN and AGE in children. There was no difference in the detection rate and
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mean viral load of Cosa-CHN between the case and control subjects. However, coinfection
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with other diarrhea-related viruses was frequent in the Cosa-CHN-positive samples from
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the case group (5/8). Further statistical analysis indicated that Cosa-CHN coinfection did
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not exacerbate the clinical symptoms of gastroenteritis. Taken together, these findings
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suggest that Cosa-CHN does not play a role in gastroenteritis. However, it should be noted
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that the viral loads were relatively low in this study. A previous study reported that
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norovirus viral loads lower than a threshold level, it should be regarded as negative; in
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other word, though the virus was detected, it was not a causal factor in the disease [26].
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This might also be the case for Cosa-CHN infection, so the possibility that a high load of
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Cosa-CHN may cause diarrhea cannot be ruled out. Moreover, specific cosavirus genotypes
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may yet be shown to be associated with specific diseases as is the case for enteroviruses.
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Further studies involving virus stability, virus isolation, animal experiments, serology and
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molecular epidemiology should be performed to evaluate the pathogenicity of different
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cosavirus species and genotypes.
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Funding information
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This work was supported by the National Natural Science Foundation of China (Grant No.
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81290345).
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Competing interest
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All authors declare no conflict of interest.
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Author contribution
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ZJD and JMY designed the experiments; JMY, YYA and LLL performed the experiments;
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JMY and YYA analyzed the results; JMY wrote the draft manuscript. ZJD revised the
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manuscript. All the authors reviewed the manuscript.
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Figure legends
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Figure 1. (a) genome organization of Cosa-CHN; (b) whole virus sequencing approach; and
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(c) protein cleavage map. Nine fragments were used to produce the final genome sequence.
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21. Yamashita T, Sakae K, Tsuzuki H, Suzuki Y, Ishikawa N, et al. (1998) Complete nucleotide sequence and genetic organization of Aichi virus, a distinct member of the Picornaviridae associated with acute gastroenteritis in humans. J Virol 72: 8408-8412. 22. Santti J, Hyypia T, Kinnunen L, Salminen M (1999) Evidence of recombination among enteroviruses. J Virol 73: 8741-8749.
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23. Simmonds P, Welch J (2006) Frequency and dynamics of recombination within different species of human enteroviruses. J Virol 80: 483-493. 24. Xing W, Liao Q, Viboud C, Zhang J, Sun J, et al. (2014) Hand, foot, and mouth disease in China, 2008-12:
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the initial PCR for HCosV and Cosa-CHN specific RT-nPCR amplicon products were in
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red and marked as "VP1" and "VP3/VP1" ,respectively.
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Figure 2. Phylogenetic analysis of Cosa-CHN sequences: (a) polyprotein amino acid
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sequences; (b) partial VP3/VP1 nucleotide sequences. The tree was constructed using the
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neighbor-joining method b ny MEGA ver. 5 with 1,000 bootstrap replicates. Sequences
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from this study are indicated by "•". Cosa-CHN formed a lineage distinct from other known
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HCosV.
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ACCEPTED MANUSCRIPT Table 1. Clinical characteristics, viral loads, and related information of eight children in the case group positive for Cosa-CHN. Duration of Patient ID
diarrhea,
Age,
Frequency of
Viral load,
diarrhea, per
copies
Sex
Area
days
Month
Coinfection
Fever
day
Vomiting
(copies/ml)
144
F
Hunan
7
8
HuCV
+
4
-
3.48×101
038
F
Hebei
3
8
-
+
061
F
Hunan
2
6
RV, AdV
+
070
M
Hunan
2
7
AstV
-
102
F
Hunan
1
3
-
N
052
M
Hunan
3
6
-
113
M
Hebei
2
15
RV
073
F
Hebei
15
4
RV
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No.
-
8.36×101
2
+
1.05×102
6
-
3.46×102
2
-
3.65×102
+
4
-
5.02×102
-
7
-
1.90×103
-
6
+
1.07×104
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Note: Duration of diarrhea indicates the time from the date of admission to the date of
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discharge from hospital. M, male; F, female; N, no data; +, present; -, absent.
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