Australian Rotavirus Surveillance Program annual report, 2007/08

This report describes the types of rotavirus strains responsible for the hospitalisation of children with acute gastroenteritis during the period 1 July 2007 to 30 June 2008, the first complete year of surveillance following introduction of rotavirus into the National Immunisation Program. Six hundred faecal samples from across Australia were examined using a combined approach of monoclonal antibody immunoassays and reverse transcription-polymerase chain reaction.

Page last updated: 28 January 2009

Carl D Kirkwood, David Cannan, Karen Boniface, Ruth F Bishop, Graeme L Barnes, and the Australian Rotavirus Surveillance Group

Abstract

The National Rotavirus Reference Centre together with collaborating laboratories Australia-wide conducts a laboratory based rotavirus surveillance program. This report describes the types of rotavirus strains responsible for the hospitalisation of children with acute gastroenteritis during the period 1 July 2007 to 30 June 2008, the first complete year of surveillance following introduction of rotavirus into the National Immunisation Program. Six hundred faecal samples from across Australia were examined using a combined approach of monoclonal antibody immunoassays and reverse transcription-polymerase chain reaction. Of the 419 confirmed as rotavirus positive, serotype G1 was the dominant serotype nationally, representing 52% of specimens, followed by serotype G2 (19.8%), serotype G9 (12.2%), and serotype G3 (11%). No serotype G4 strains were identified. All G1, G3 and G9 strains assayed for P genotype contained the P[8] genotype, while all G2 strains contained the P[4] genotype, except one G2 strain which possessed a P[8]. Uncommon rotavirus genotypes, G8 (n=2) and P[9] (n=2) were identified during this study period. There was no evidence of unexpected changes in serotype distribution during the first 12 months of rotavirus vaccine use in the National Immunisation Program. Commun Dis Intell 2008;32:425–429.

Top of page

Introduction

Rotavirus vaccine was introduced into the National Immunisation Program of Australia for all young infants from 1 July 2007. This is aimed to decrease the huge social and economic burden of rotavirus disease in Australia, which accounts for up to 50% of childhood hospitalisations for diarrhoea in Australia, and which represents 10,000 children hospitalised each year,1 costing an estimated $30 million in direct costs.2

The 2 rotavirus vaccines, Rotarix® [GlaxoSmithKline] and RotaTeq® [Merck], have both been demonstrated to be safe and highly effective in the prevention of severe diarrhoea and hospitalisation due to rotavirus infections during large-scale phase III clinical and efficacy trials, each involving over 60,000 children worldwide.3,4 In Australia, the state and territory health departments each made independent decisions on which vaccine to select; Victoria, South Australia, and Queensland selected RotaTeq®, while New South Wales, Western Australia, the Northern Territory, Tasmania and the Australian Capital Territory selected Rotarix®.

The Australian Rotavirus Surveillance Program has been reporting the changing annual pattern of dominant serotypes in the Australian population since 1999. Over this period our results highlight the diversity of rotavirus strains capable of causing disease in children, and provide the baseline information of the changing pattern of circulating strains, prior to vaccine introduction.5–7

The impact of these 2 widely used vaccines on the natural pattern of circulating rotavirus strains is unknown and difficult to predict, given the different components of each vaccine. Continuing serotype surveillance should identify the effects that each vaccine program has on circulating strains—in particular, whether changes occur in serotype incidence and whether increased proportions of rare or uncommon types result.

In this report we describe the surveillance and characterisation of rotavirus strains causing the annual epidemics of severe diarrhoea in young children in Australia for the period 1 July 2007 to 30 June 2008, the first 12 months in which rotavirus vaccine was available through the immunisation program.

Top of page

Methods

Rotavirus positive specimens detected by enzyme immunoassay (EIA) or latex agglutination in collaborating laboratories were collected, stored frozen and forwarded to Melbourne together with relevant age and sex details. Specimens were then serotyped using an in-house monoclonal antibody (MAb) based serotyping EIA. The EIA employed a panel of MAbs specific for the major glycoprotein VP7 of the outer capsid of the 5 major group A human rotavirus serotypes (G1, G2, G3, G4 and G9).8 Strains which could not be assigned a G serotype were genotyped by using a hemi-nested multiplex reverse transcription/polymerase chain reaction (RT-PCR), using G specific oligonucleotide primers.9 P genotypes were determined by using a hemi-nested multiplex RT-PCR assay.10

Top of page

Results

Number of isolates

A total of 600 specimens were received for analysis from Melbourne, Victoria and the collaborating centres in Western Australia, the Northern Territory, New South Wales and Queensland (Table). Specimens were not obtained from either South Australia or Tasmania. Four hundred and nineteen specimens were confirmed as rotavirus positive using our in-house EIA assay. The remaining 181 specimens contained either insufficient specimen for testing, or the specimens were not confirmed to be positive for rotavirus and were not analysed further.

Table. Rotavirus G serotypes in Australia, 1 July 2007 to 30 June 2008

Centre
Total number Serotype
G1 G2 G3 G4 G9 mix NR
% n % n % n % n % n % n % n
New South Wales
Sydney (POW)
6
50
3
0.0
0
16.7
1
0.0
0
16.7
1
0.0
0
16.7
1
Sydney (Westmead)
33
39.4
13
27.3
9
21.2
7
0.0
0
0.0
0
3.0
1
9.1
3
Northern Territory
Alice Springs
37
0.0
0
40.5
15
0.0
0
0.0
0
46
17
0.0
0
13.5
5
Darwin
18
0.0
0
61.1
11
11.1
2
0.0
0
22.2
4
0.0
0
5.6
1
Western Diagnostic (NT)
8
25
2
62.5
5
0.0
0
0.0
0
0.0
0
0.0
0
12.5
1
Queensland
Brisbane
26
15.4
4
34.6
9
27.0
7
0.0
0
11.5
3
0.0
0
11.5
3*
Victoria
Melbourne
82
64.6
53
5
6.1
18.3
15
0.0
0
3.7
3
0.0
0
7.3
6
Western Australia
PathWest WA
134
68.7
92
11.2
15
3.7
5
0.0
0
11.9
16
0.0
0
4.5
5*
Perth
48
85.4
41
2.1
1
0.0
0
0.0
0
4.2
2
2.1
1
6.2
3
Western Darwin Pathology
27
0.0
0
48.2
13
33.3
9
0.0
0
18.5
5
0.0
0
0.0
0
Total
419
52.0
218
19.8
83
11.0
46
0.0
0
12.2
51
0.5
2
4.5
19

An additional 181 specimens were omitted from analysis due to insufficient sample or because the specimen was not confirmed to be rotavirus positive.

* Two samples were identified as genotype G8 (PerthWest and Brisbane).

Top of page

Age distribution

The overall age distribution of children with acute rotavirus gastroenteritis is depicted in the Figure. In the reporting period, 11% of cases were from infants 0–6 months of age, 17.9% were from infants 7–12 months of age, 28.4% from patients 13–24 months of age, and 13.1% from patients 25–36 months of age. Overall, 86.9% of samples were from children aged 5 years or less.

During the study period, slightly more specimens from male than female children (n=317 vs. 247) were obtained for analysis.

Figure. Cases of rotavirus, Australia, 1 July 2007 to 30 June 2008, by age group

Cases of rotavirus, Australia, 1 July 2007 to 30 June 2008, by age group

Serotype distribution

The rotavirus serotypes identified in Australia from 1 July 2007 to 30 June 2008 are shown in the Table. Serotype G1 was the most common, representing 52% of all specimens, and was identified in Melbourne, Sydney, Perth and Brisbane, however only two of 90 rotaviruses identified in the Northern Territory were G1, both in Darwin. G1 was the dominant type in Melbourne, Sydney and Perth. Serotype G2 was the second most common type nationally, and represented 19.8% of specimens. It was identified in eight of the 10 collaborating centres and was the dominant type in Darwin and Brisbane. Strains belonging to serotype G9 were the third most common type identified, representing 12.2% of specimens. G9 was found in eight of the 10 centres, and was dominant in Alice Springs, prior to this surveillance period. This was probably related to the large rotavirus gastroenteritis outbreak which occurred in early 2007 in Alice Springs. Serotype G3 strains were identified in 7 centres during the study, and represented 11% of the total strains identified. No serotype G4 strains were identified in any centre. Two genotype G8 strains were identified during the study, one in Perth and one in Brisbane.

P genotype was determined for 116 of the rotavirus positive samples. All of the 25 G1 strains analysed were genotyped as P[8]. Similarly, all of the G3 and G9 strains analysed were also genotyped as P[8] (n=21 and 23, respectively). Thirty-eight of the 39 G2 strains analysed were associated with P[4]: 1 sample was typed as G2P[8]. Two G non-typeable strains were found to possess the P[9] VP4 gene.

Less than 0.5% of the rotavirus samples contained multiple serotypes. In 4.5% of the samples a serotype was not identified. The latter could be samples with virus numbers below the detection limits of our typing assays, or could have contained inhibitors in extracted RNA that prevent the function of the enzymes used in RT and/or PCR steps. Future studies will include further characterisation of the genes encoding the outer capsid proteins of these strains.

Faecal specimens were received from 12 children who developed gastroenteritis with 2 weeks of being vaccinated. No vaccine virus was identified in any of the cases, and in all cases wild type rotavirus strains were detected.

Top of page

Discussion

In this report covering the period 1 July 2007 to 30 June 2008, we describe the annual epidemics and geographic distribution of the rotavirus types causing disease in Australian children during the first 12 months after national rotavirus vaccine introduction. Serotype G1 remained the dominant serotype nationally, comprising 52% of all strains characterised. It continues to be the dominant type on both sides of the country, in particular in Melbourne, Sydney and Perth, and was a minor strain in the Northern Territory. This survey continues to highlight the importance of serotype G1 as a major cause of disease in Australian children.

As noted in previous reports, multiple serotypes continue to co-circulate within the Australian population causing significant disease.5–7 This year, G2, G3 and G9 were each identified in at least 7 locations during 2007–2008 and were all identified in greater than 10% of specimens.

The prevalence of G2 strains has increased during this survey, with G2 being the predominant type identified in the Northern Territory and Brisbane. During the 2004/05 and 2005/06 surveys G2 was a minor strain, identified in less than 2% of strains.5,6 G2 has slowly increased in prevalence in Sydney and Melbourne, being the second most common strain during the 2006/07 period.7 This year G2 predominated in the Northern Territory for the first time since it was responsible for a large outbreak of gastroenteritis in January 2004.11

In each of the G1, G3 and G9 strains analysed for VP4 genotype, the expected association with the P[8] VP4 protein was identified. Thus G1P[8], G3P[8] and G9P[8] combinations were the predominant strains identified in children during the current surveillance period similar to what is seen worldwide.12,13 The G2 strains showed the expected association with the P[4] VP4 genotype, with 1 exception, the unusual G2P[8] strain that was identified in Brisbane. This is the first G2P[8] strain reported in Australia.

Both rotavirus vaccines used in Australia, RotaTeq and Rotarix have been shown to provide excellent protection against severe rotavirus gastroenteritis in large Phase III safety and efficacy trials.2,3 RotaTeq® is a live attenuated bovine-human pentavalent vaccine. It contains rotavirus reassortants G1, G2, G3, G4 and P1[8] derived from rotaviruses infecting human and bovine species, which provides serotype specific protection against the most common rotavirus types. Rotarix® contains a live attenuated strain of human rotavirus (G1P[8]). Protection involves production of both specific and cross reactive antibodies, and has been demonstrated against serotypes G1, G3, G4 and G9. In a comparison of rotavirus types identified, based on vaccine usage in the various states, differences in the prevalence rates of G2, G3 and G9 were seen. G2 and G9 strains were more prevalent in states using Rotarix, whereas G3 strains were more prevalent in states using RotaTeq. These differences do not necessarily imply lack of protection by either vaccine against a particular type, but rather highlight the variation that can occur due to natural annual fluctuation in rotavirus strain prevalence.

Top of page

Uncommon rotavirus types continue to be of worldwide interest because of the possible impact they may have on rotavirus vaccine programs. This year, 2 uncommon types have been identified in Australian children. Strains exhibiting a genotype G8 VP7 protein were identified in Perth and Brisbane, extending the previous identification of G8 in 2006–07 in Darwin. This continues the sporadic identification of G8 strains as a cause of acute gastroenteritis in Australian children.7,14 The second uncommon type identified during this survey was the P[9] VP4 genotype in 2 strains. These strains were identified in Darwin, and represent the first report of P[9] in Australia. Previous reports of P[5] have been associated with G6 in the United States of America and Hungary, and G12 in Japan and Thailand.12,13 Thus these reports of uncommon strains continue to highlight their low level existence in Australian children.

Prior to rotavirus vaccine introduction approximately 70% of clinical disease occurred among children less than 24 months of age.7 During the previous survey (2006/07) 16% of faecal specimens were received from children admitted to hospital aged 0–6 months, and 23.9% of specimens were from infants aged 7–12 months. In comparison, the age distribution of children admitted to hospital during the first 12 months after implementation of the rotavirus vaccination programs has seen a slight reduction in the proportion of 0–6 and 7–12 month age groups affected, with 13% of specimens derived from infants aged 0–6 months, and 21% of specimens from infants aged 7–12 months. The potential impact of rotavirus vaccination is illustrated by the finding that no rotavirus positive specimens were received from infants aged 0–6 months in Darwin, despite faecal specimens being collected for serotype analysis from 54 children in Darwin during this survey period.

There have been no unexpected changes in the serotype distribution of rotavirus types causing disease in Australian children since the introduction of vaccination program nationwide. The rotavirus typing results from this survey, together with those of previous years, highlight the unpredictable nature of changes in the prevalence of rotavirus strains across Australia. In addition, the identification of rare or uncommon VP7 and VP4 genotypes further illustrate the diversity of strains capable of causing severe disease in Australian children. Understanding the fluctuations in rotavirus serotypes, using multicentre national surveillance, will provide valuable insight into vaccine efficacy over the next 3–5 years.

Top of page

Acknowledgements

The Australian Rotavirus Surveillance Program is supported by grants from the Australian Government Department of Health and Ageing, GlaxoSmithKline and CSL.

Dr Kirkwood is supported by an RD Wright Fellowship, National Health and Medical Research Centre.

Rotavirus positive specimens were collected from numerous centres throughout Australia. The significant time and effort involved in the collection, storage, packaging, compiling data and forwarding of specimens was much appreciated.

The National Rotavirus surveillance group includes:

New South Wales

Prof W Rawlinson, Dr C McIver and members of the Virology Division, Prince of Wales Hospital

Dr A Kesson and members of the Microbiology Department, The Children's Hospital at Westmead

Northern Territory

Dr P Southwell and members of the Microbiology Department, Royal Darwin Hospital, Casuarina

Dr M Leung, Ms H Reed and members of the Department of Microbiology, Western Diagnostic Pathology, Northern Territory and Western Australia

Mr J McLeod and members of the Microbiology Department, Alice Springs Hospital, Alice Springs

Top of page

Queensland

Dr M Lyon, Queensland Health, Forensic and Scientific Services, Herston

Dr M Nissen, Infectious diseases, Royal Children's Hospital, Herston

Victoria

Dr R Alexander and members of the Virology Department, Royal Children's Hospital, Parkville

Western Australia

Dr K Lindsay and members of the Virology Department, Princess Margaret Hospital for Children, Subiaco

Dr D Smith, Dr G Harnett and members of Division of Microbiology, PathWest LM.

The Queen Elizabeth Medical Centre, Nedlands

Author details

Dr Carl D Kirkwood, Senior Research Fellow

Mr David Cannan, Research Assistant

Ms Karen Boniface, Research Assistant

Professor Ruth F Bishop AO, Senior Principal Research Fellow

Professor Graeme L Barnes, Senior Principal Research Fellow

National Rotavirus Reference Centre, Murdoch Childrens Research Institute, Royal Children's Hospital, Flemington Road, Parkville, Victoria, 3052.

Corresponding author: Dr Carl Kirkwood, Enteric Virus Research group, Room SW834, 8th floor AP Building, Murdoch Childrens Research Institute, Royal Children's Hospital, Flemington Road, PARKVILLE VIC 3052. Telephone: +61 3 8341 6439. Facsimile: +61 3 8341 6449. Email: carl.kirkwood AT mcri.edu.au

Top of page

References

1. Carlin J, Chondros P, Masendycz P, Bugg H, Bishop R, Barnes G. Rotavirus infection and rates of hospitalisation for acute gastroenteritis in young children in Australia, 1993–1996. Med J Aust 1998;169:252–256.

2. Galati JC, Harsley S, Richmond P, Carlin JB. The burden of rotavirus-related illness among young children on the Australian health care system. Aust N Z J Public Health 2006;30:416–421.

3. Vesikari T, Matson DO, Dennehy P, Van Damme P, Santosham M, Rodriguez Z, et al. Safety and efficacy of a pentavalent human-bovine (WC3) reassortant rotavirus vaccine. N Engl J Med 2006;354:23–33.

4. Ruiz-Palacios GM, Perez-Schael I, Velazquez FR, Abate H, Breuer T, et al. Safety and efficacy of an attenuated vaccine against severe rotavirus gastroenteritis. N Engl J Med 2006;354:11–22.

5. Kirkwood CD, Bogdanovic-Sakran N, Cannan D, Bishop RF, Barnes GL. National Rotavirus Surveillance Program, annual report: 2004/2005. Commun Dis Intell 2006;30:120–123.

6. Kirkwood CD, Cannan D, Bogdanovic-Sakran N, Bishop RF, Barnes GL; National Rotavirus Surveillance Group. National Rotavirus Surveillance Program annual report, 2005–06. Commun Dis Intell 2006;30:434–438.

7. Kirkwood CD, Cannan D, Bogdanovic-Sakran N, Bishop RF, Barnes GL. Australian Rotavirus Surveillance Program, 2006–07. Commun Dis Intell 2007;31:375–379.

8. Coulson BS, Unicomb LE, Pitson GA, Bishop RF. Simple and specific enzyme immunoassay using monoclonal antibodies for serotyping human rotaviruses. J Clin Microbiol 1987;25:509–515.

9. Gouvea V, Glass RI, Woods P, Taniguchi K, Clark HF, Forrester B, et al. Polymerase chain reaction amplification and typing of rotavirus nucleic acid from stool specimens. J Clin Microbiol 1990;28:276–282.

10. Gentsch JR, Glass RI, Woods P, Gouvea V, Gorziglia M, Flores J, et al. Identification of group A rotavirus gene 4 types by polymerase chain reaction. J Clin Microbiol 1992;30:1365–1373.

11. Kirkwood C, Bogdanovic-Sakran N,Bishop R, Barnes G. Report of Australian Rotavirus Surveillance Program, 2003–2004. Commun Dis Intell 2004;28:481–485.

12. Santos N, Hoshino Y. Global distribution of rotavirus serotypes/genotypes and its implication for the development and implementation of an effective rotavirus vaccine. Rev Med Virol 2005;15:29–56.

13. Gentsch JR, Laird AR, Biefelt B, Griffin DD, Banyau K, Ramachandran M, et al. Serotype diversity and reassortment between human and animal rotavirus strains: implications for rotavirus vaccine programs. J Infect Dis 2005;192:S146–S159.

14. Cooney MA, Gorrell RJ, Palombo EA. Characterisation and phylogenetic analysis of the VP7 proteins of serotype G6 and G8 human rotaviruses. J Med Microbiol 2001;50:462–467.


Related Links

Communicable Diseases Intelligence subscriptions

Sign-up to email updates: Subscribe Now

This issue - Vol 32 No 4, December 2008