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Transcript
HHV-6 The disease and Panbio product training Overview • First isolated in 1986 from patients with AIDS • The main clinical syndrome associated with the virus, roseola infantum, was first reported in 1913 • It wasn’t until 1988 that the link between HHV-6 and roseola infantum was established.[1] • Ubiquitous virus which causes disease in both normal and immunocompromised individuals • HHV-6 is a viable candidate as a possible etiological agent in multiple sclerosis. Infectious Agent • Belongs to the Betaherpesvirus subfamily and genetically similar to HHV-7 and CMV – cross reactivity between HHV-6 and CMV is quite common[2]. • Two distinct variants - HHV-6A and HHV-6B – Can be differentiated using monoclonal antibodies and PCR • Incubation period about 10 days Epidemiology • Approximately 90% of normal children are infected during infancy, with the peak age of 6-9 months.[1] • In Western populations most children are infected by the age 3 years, and the majority of these with HHV6B.[2] • Transmission via saliva from infected individuals, blood transfusion and organ transplantation.[4] • Incidence is greatest in Spring Pathogenesis • CD4+ T-lymphocytes are the preferential cell for HHV6 to infect, with the surface marker CD46 acting as part of a co-receptor for infection.[5] This in turn results in a number of significant effects on the immune system. • HHV-6 infection persists for an extended period, with the virus able to establish latency in a number of different cells and organs. Clinical Notes Infection in childhood • Exanthema subitum (Roseola infantum or sixth disease) – Occurs in infants – High fever that lasts 3-5 days – Maculopapular rash (Physicians can mistake these signs for allergic reactions to antibiotics.[1] ) – Associated with febrile convulsions in 12-15 month old children. – Febrile form usually self-limiting and does not require specific therapeutic intervention Clinical infection Immunocompromised patients • Reactivation of HHV-6 infection may result in fever, skin rash, pneumonitis, encephalitis and even bone marrow suppression. • Reactivation in bone marrow transplant patients has a particularly high incidence of 48%.[1] • High frequency of HIV-infected patients that suffer from HHV-6 reactivation resulting in pneumonitis and encephalitis. • HHV-6 has been increasingly associated with conditions such as MS and malignancies such as Hodgkin’s disease, non-Hodgkin’s lymphoma, acute lymphoblastic leukaemia, oral carcinoma and cervical carcinoma. Antibody Response • Although many newborns maternally acquire HHV-6 antibodies they become seronegative by 6 months. • Antibody levels may be elevated in patients with infectious mononucleosis (IM), chronic fatigue, Hodgkin's disease & oral and cervical carcinoma. • Primary infection – IgM detectable 5-7 days after febrile phase of Roseola – IgG appears 7-10 days after the febrile phase of Roseola and usually persists for life. Diagnosis • Clinically may be confused with measles and rubella because of similar rash. • Laboratory confirmation essential to ensure effectiveness of measles and rubella surveillance programs. • Diagnostic tests – – – – IFA Viral isolation PCR ELISA Why Test for HHV-6? • • • • • • Ubiquitous virus that causes a wide range of disease. Because it is common, immunocompromised patients are more likely to come into contact with individuals who are suffering from primary HHV-6 infection. Transplant patients who are being medicated against graft rejection are particularly susceptible. HIV-infected individuals are also susceptible. Whilst HHV-6 usually causes a benign, self-limiting disease in children, there are a number of cases that progress to serious life-threatening states of the disease. As IgM to HHV-6 can cross react with a number of other viral antigens such as CMV and EBV, testing of both HHV-6 IgG and IgM affords the physician with a clearer picture as to whether an individual preparing to undergo transplantation is at risk of reactivation or primary infection. Diagnostic Tests • Virus isolation – has been successful in primary infections, usually when rash is present. – time-consuming • PCR – useful for variant discrimination – useful in viremic part of disease - usually first 3-4 days after illness only • IFA – useful for confirmation and small scale testing • ELISA – for IgG and IgM antibodies – use in conjunction with IFA for confirmation Diagnostic Tests Virus Isolation PCR IgM ELISA or IFA IgG ELISA or IFA Panbio HHV-6 IFA Products • • • • • HHV-6 IgG IFA kit HHV-6 IgG IFA kit HHV-6 IgM IFA kit HHV-6 IgM IFA kit HHV-6 IFA Slides 120T 40T 120T 40T 10x10well Cat# I-HV601G Cat# I-HV603G Cat# I-HV601M Cat# I-HV603M Cat# I-HV601X Panbio HHV-6 IgG and IgM IFA • • Bright green fluorescent staining = positive Fluorescent staining pattern of HHV-6 infected cells is variable. – Depending on the cell’s stage of infection, the fluorescent pattern can vary from a small portion of the infected cell fluorescing to the whole cell fluorescing. – Fluorescence can also range from granular to homogeneous. • To provide an internal control, each well contains both HHV6 infected and uninfected cells. Preparation of the slide in this manner is intentional. – Uninfected cells, stained red by the counterstain, provide a contrasting background. – Infectivity of the cells ranges from 20% - 60%. • Absence of specific fluorescent staining of the infected cells denotes a negative reaction. HHV-6 IgG IFA performance • Dr. Theo Sloots, Clinical Virology Research Unit, Sir Albert Sakzewski Virus Research Centre (SASVRC), Royal Children’s Hospital, Qld, Australia. • Sample population 1. Blood donors (n=23) 2. Acute sera from children with proven HHV-6 infection (n=22) 3. Convalescent sera from children with proven HHV-6 infection (n=35) • Agreement of 95% (76/80) Panbio HHV-6 IgM ELISA • HHV-6 IgM ELISA Cat # E-HV601M • For the presumptive qualitative detection of IgM to HHV-6 in serum as an aid in the clinical laboratory diagnosis of primary of reactivated HHV-6 infection in patients presenting clinical symptoms consistent with HHV-6 infection. Panbio HHV-6 IgM ELISA Performance • Package insert • Study 1 – 149 serum samples (98 Aust blood donors and 40 positives characterised by in-house IFA) – Serological sensitivity = 52.5% – Clinical specificity = 87.8% – Relative agreement = 77.5% • Cross reactivity – Cross reactivity observed with CMV and EBV primarily Panbio HHV-6 IgG ELISA • HHV-6 IgG ELISA Cat # E-HV601G • For the qualitative detection of IgG to HHV-6 in serum as an aid in diagnosis of recent or past exposure to HHV-6 • Paired sera required to determine recent infection if using IgG alone Panbio HHV-6 IgG ELISA Performance • Sloots et al., 1996, J. Clin. Micro – Sensitivity 99.8%, Specificity 98.8% • Package insert – 212 serum samples characterised by public hospital lab’s in-house IFA – Clinical sensitivity = 97.4% – Serological specificity = 86.0% – Serological agreement = 94.3% Comments from Dr Sloots • • • • The kit was easy to use and reagents were adequate Good cell numbers were present per well Strong apple-green fluorescence was present at 4+ The fluorescence of positive reactions (4+ to 1+) was easily discriminated from the negative reaction • The percentage of infected cells per field was high (70%) Further performance data is found in the HHV-6 IgG IFA package insert Promotional Resources • Clinical notes sheet • Colour brochure – in process of being updated • Publications – General – Panbio HHV-6 IgG ELISA References 1. 2. 3. 4. 5. 6. 7. 8. Abdel-Haq, N.M., Asmar Basim, I. (2004). Human herpesvirus 6 (HHV6) infection. The Indian Journal of Pediatrics. 71(1):89-96. Irving, W.L., et al. (1990). Dual antibody rises to cytomegalovirus and human herpesvirus type 6: frequency of occurrence in CMV infections and evidence for genuine reactivity to both viruses. Journal of Infectious Diseases. 161(5): 910-916. Caserta, M.T., Mock, D.J., Dewhurst, S. (2001). Human herpesvirus 6. Clinical Infectious Diseases. 33(6): 829-833. Okuno, T., et al. (1989). Seroepidemiology of human herpesvirus 6 infection in normal children and adults. Journal of Clinical Microbiology. 27(4): 651-653. Lau, Y.L., et al. (1998). Primary human herpes virus 6 infection transmitted from donor to recipient through bone marrow infusion. Bone Marrow Transplant. 21(10): 1063-1066. Santoro, F., et al. (1999). CD46 is a cellular receptor for human herpesvirus 6. Cell. 99(7): 817-827. Steeper, T.A., et al. (1990). The spectrum of clinical and laboratory findings resulting from human herpesvirus-6 (HHV-6) in patients with mononucleosis-like illnesses not resulting from Epstein-Barr virus or cytomegalovirus. American Journal of Clinical Pathology. 93(6): 776-783. Dockrell, D.H., Paya, C.V. (2001) Human herpesvirus-6 and –7 in transplantation. Reviews in Medical Virology. 11(1): 23-36.
