Friday, April 5, 2019
Proposal to Cease Testing Blood Donations for CMV
Proposal to Cease Testing simple eye Donations for cytomegalo virus side PublicExecutive summary (200 words)In response to SaBTO recommendations for replacing cytomegalovirus sero controvert cellular roue fragments with leucodepleted alliance components, an executing project has been established pending approval from the Board. The proposed implementation date of January 2018 is strikeed a realist timeframe for this approach. Communication with clinicians indicates the borrowing of leucodepleted components as cytomegalovirus safe, replacing the selection of cytomegalovirus seronegative components. Information has been obtained regarding international practices and substance abuse of leucodepletion with respect to cytomegalovirus.This opus sets out key information on the proposed replacement of cytomegalovirus seronegative stock products with leucodepleted channel products, provides recommendations of the optimal scheme to achieve this, and takes into consideration unhur ried groups that may be affected.Action requested (bulleted list)The Board is asked toNote the implementation plans for the introduction of cytomegalovirus safe filiation productsApprove the proposal to cease occupation of all cytomegalovirus seronegative subscriber line products that undergo leucodepletion and consider these products as cytomegalovirus safeApprove the proposal to continue the takings of cytomegalovirus seronegative red cell and descent platelet components for intra-uterine transfusions and neonatesApprove the proposal to continue the production of cytomegalovirus seronegative granulocyte components for cytomegalovirus seronegative patientsApprove the proposal to continue the production of cytomegalovirus seronegative blood components for seronegative and seropositive pregnant women that require transfusions throughout pregnancyAgree the recommendation to continue to implement CMV PCR as a cover version method for previous(predicate) detection for all hae mopoietic stem cell and solid electric organ graft recipientsPurpose of root word (1 paragraph)For over 30 years, there has been an ongoing debate regarding the use of CMV seronegative blood components versus the use of leucodepleted blood components. To date, the use of CMV seronegative blood products has been enforced to suppress the jeopardize of transfusion-transmitted cytomegalovirus in patients considered at venture. Leucodepletion has been performed on all blood products in the UK since 1999. This paper provides an overview on the use of CMV seronegative blood products in resemblance to the use of leucodepleted blood components. This paper provides an measure outment of patient groups that ar considered at endangerment of CMV and considers advantages to ceasing of CMV interrogation in the UK.Backgroundcytomegalovirus (CMV) is a pervasive, cell-associated prototypic virus that is a member of the betaherpesvirus subfamily (Ziemann and Hennig, 2014 Ljungman, 2004). CMV mostly causes asymptomatic infection or mononucleosis-like-infection in an immunocompetent host however, in an immunocompromised host it lavatory result in chronic and persistent infection with devastating outcomes (Seed et al., 2015). Patient groups that ar considered at risk of life-threatening transfusion-transmitted CMV infection involves CMV seronegative patients undergoing haematopoietic stem cell transplantation and solid organ transplantation, low birth weight and premature neonates, foetuses that require intrauterine transfusion, CMV seronegative pregnant women, and passing immunocompromised patients, such as those with malignant disease (Ziemann and Hennig, 2014 SaBTO, 2012).CMV infection is frequently encountered throughout childhood and an estimated 50 60% of the adult population in the United Kingdom (UK) ar CMV positive (SaBTO, 2012). CMV infection mint be transmitted both horizontally and vertically (Crough and Kannah, 2009). Horizontal transmission occurs through contact with body fluids, such as urine and saliva, sexually through genital secretions, blood transfusion, and haemopoietic stem cell and organ transplant (SaBTO, 2012 Sia and Patel, 2000). Vertical transmission occurs from mother to child, via deliverance and breast take out (Crough and Kannah, 2009). Additionally, congenital CMV infection is highly predominant and may arise through a primordial maternal infection during pregnancy (Crough and Kannah, 2009).Following exposure to CMV and the initial infection, the virus remains in a dormant state (Ljungman, 2004). Seroconversion of the host occurs between 6 8 weeks and mounts an immune response, producing CMV particular proposition immunoglobulin (IgG) (Seed et al., 2014). In the UK, there is an estimated seroconversion rate of 1% per annum (SaBTO, 2012). CMV therefore has a window period, in which there may be underlying viremia and high viral load (Liberman et al., 2011). Subsequently, a CMV seropositive individual i s considered to have been infect, whilst at the same time considered potentially infectious due to the life-long persistence of the virus (SaBTO, 2012).Transfusion-transmitted CMV infection is regarded as a potential threat to the safety and sufficiency of the blood tot up for a multitude of reasons (Roback, 2002). Firstly, transfusion-transmission of CMV that is present in blood and blood components can result in the infection of nave recipients (Ziemann and Hennig, 2014 Ljungman, 2004). Secondly, transfusion-transmitted CMV is acknowledged as a primary source of infection, in which sponsor infectivity is an underlying reason, that may result in CMV disease (Ljungman, 2004). Thirdly, CMV seropositive recipients that are exposed to blood products containing CMV may cause reactivation of the latent virus or reinfection from a new strain (Ziemann and Hennig, 2014 Ljungman, 2004). However, the risk of transfusion-transmitted CMV infection has been evidentiaryly ignored through the implementation of leucodepletion and production of specific CMV negative blood and blood products (Ziemann and Hennig, 2014).Since November 1999, all blood products (un slight state otherwise) produced by the UK blood service are leucodepleted (Guidelines for the Blood Transfusion function in the United Kingdom, 2013). Initially, this was a response taken to reduce the risk of var. Creutzfeldt-Jakob (vCJD) disease in blood transfusions however, this risk decrease strategy has proven beneficial in extra areas of transfusion science and blood safety (Guidelines for the Blood Transfusion Services in the United Kingdom, 2013). The UK specification for leucodepletion is more than 90% of leucocyte-depleted components should contain less than 1 x 106 leucocytes and more than 99% of components should contain less than 5 x 106 leucocytes (SaBTO, 2012). The specification for 99% of components is regarded as the level in which blood components are deemed CMV safe (SaBTO, 2012).Leucodeple tion has considerably reduced the risk of transfusion-transmitted CMV, to a level that mirrors the selection of CMV negative blood products (Ljungman, 2004 Bowden et al., 1995). However, it has yet to be shown to what extent the techniques are comparable and how this may affect patient groups considered at risk of CMV infection (Ljungman, 2004). It is important to note that whilst leucodepletion removes most white cells from blood products, it is not 100% impelling (Kumar, 2006). Therefore, there is a residual risk of CMV transmission in blood products of recently infected donors (Kumar, 2006). This occurs in the window period of the virus from 6 8 weeks to 1 year following seroconversion, in which the virus may be present in the remaining plasma or white cells (SaBTO, 2012 Ziemann et al., 2010 move and Roback, 2007).CMV transmission can occur in both donors that have an active infection, including primary or reactivated, or latent infection (Azevedo, 2015). The leading mechanism of transfusion-transmitted CMV infection is through mononuclear cells that are believed to harbour a latent infection (Ljungman, 2004). CMV is thought to persist in circulating monocytes, in which an estimated 1 in 10,000 and 1 in 100,000 peripheral blood monocular cells carry CMV (SaBTO, 2012). Pennington et al (2001) conducted a study that provided evidence to suggest that leucodepletion filters are highly effective in removing mononuclear cells and may reduce CMV levels to 0.1 viral copies per mL in leucodepleted blood. Furthermore, blood products that have been leucodepleted are monitored continuously, utilize flow cytometry, to esteem efficiency (SaBTO, 2012). Moreover, the prospect of having a component issued that contains a leucocyte count above the UK specification can be calculated (SaBTO, 2012).In regards to testing for transfusion-transmitted CMV, there are two main methods that are used. This includes serological testing and Nucleic Acid Technology (NAT) testing (SaB TO, 2012). Serological testing involves the use of antibody screening which is accomplished through the use of enzyme immunoassay (EIA) tests that detect total CMV antibody (Ross, 2011). Screening for CMV infection using serology is the most prevalent method used and is based on the agglutination principle (Ross, 2011 Ljungman, 2004). The method offers several advantages as it is fast, highly sensitive, and highly specific, constituting an ideal screening test (Ross, 2011). This method, however, is associated with two key limitations. Firstly, the window period presents a contend in regards to activation of the primary infection and seroconversion (Ljungman, 2004). Secondly, there is a risk of obtaining false negative screening results (Ljungman, 2004). Therefore, there is a risk that CMV may be transmitted via a CMV seronegative component (SaBTO, 2012).In addition to serology, NAT testing is used to detect CMV DNA and subsequent infection (Ross, 2011). several(prenominal) qualitat ive and quantitative assays are available for this method (SaBTO, 2012). This screening method is associated with variation in the esthesia and specificity of available assays (Roback et al., 20032001). Studies have highlighted inter-laboratory variation for samples containing low viral load (Pang et al, 2009 Wolff et al., 2009). As a result, a CMV DNA reference has been developed for comparison of results when sensitivity is a challenge (Ross, 2011).To produce a deliver of CMV negative blood and blood components, several donations are screened each year. Overall, an estimated 25 40% of donors are CMV antibody positive, dependent on age. The production and use of CMV negative blood components forms a significant undertaking for the blood service. According to the pass over released by the Advisory Committee on the Safety of Blood, Tissues, and organs (SaBTO) in March 2012, in the last 5 years, the number of CMV negative platelets and red cells has increased. The report notes tha t NHSBT charge 7.76 for CMV negative red cells and platelets, covering the inventory and screening costs. This amounts to a total of 2.5 one million million million per annum, in which 230,000 is dedicated to pheresis platelets and 2,270,000 to red cells.The number of donations that are screened is greater than the number of donations that are issued as CMV negative. In addition, not all donations screened go forth deliver a negative result. Subsequently, it has been proposed that the use and production of CMV negative components is reviewed. SaBTO recommends the use of a single inventory and accepting leucodepleted blood products as CMV safe. This is outlined in section 6.Proposal6.1 This proposal has been written to ask the blood centre to consider ceasing CMV testing for an agreed list of blood products and in its replacement, support the use of leucodepleted blood components that are considered CMV safe.6.2The proposal of ceasing CMV testing for the replacement of leucodeplete d components that are considered CMV safe is associated with several advantages. arsenal managementManagement of a single inventory would offer an advantage to blood banks and hospitals. This would be a preferred method to the current used for ease of access. NHSBT must ensure CMV negative components are available across the country on multiple NHS sites. To achieve this, NHSBT spend approximately 95,000 n the delivery of CMV negative components.WastageThe Belgian Blood Service have produced a report that states implementation of pathogen reduction in platelets to inactivate CMV may result in an overall decrease in the wastage of platelets. A 1.5% reduction is estimated, which would result in a saving of 0.22 million.Improved compliance with safety initiativesReduction in the wastage of blood products and implementation of a single inventory would enable the target of 80% platelets by apheresis to be met sooner. Furthermore, this would support transfusion related acute lung injury ( TRALI) prevention, as the number of male platelet donors would increase due to enhanced recruitment strategies. This would further enable costs of HLA antibody screening of potential effeminate platelet donors to be avoided.Reduction in hospital blood bank workloadBecause of the removal of CMV seronegative components, the workload in hospitals and blood banks would decrease. Staff would no longer have to spend time parliamentary procedure or checking platelets as CMV negative components. This would have a direct positive impact on the stock management. Staff that may potentially be free from the responsibility associated with CMV negative products allow be able to invest their time elsewhere, to improve the efficiency of the blood service.Reduction in clinical errorsThe Serious Hazards of Transfusion (SHOT) have describe from 2000 to 2010, 1040 reports were filed stating special requirements were not met. Of these, 83 were attri just nowed to the inappropriate selection of blood components that were not CMV negative. 65 were attributed to selection of blood components that were both CMV negative and irradiated components. However, none of these cases reported CMV transmission.6.3The proposed implementation date of this project is January 2018. Further clinical guidance is to be requested from SaBTO who will instruct in the implementation plan of this proposal.6.4Consideration must be given to specific patient groups that are considered at risk of CMV infection. This includesHaematopoietic stem cell transplant patientsLeucodepleted blood products can be used for all patient groups post haemopoietic stem cell transplantationPatients receiving transfusions and may need a transplant also may receive leucodepleted productsCMV PCR should be used to assess CMV infection for patient groups to enable early detection and treatmentIntra-uterine transfusions and neonatesCMV negative components should be provided for intra-uterine transfusions and neonates (up to 28 da ys post expected due date)All blood products produced at a reduce size for neonates should be CMV seronegativePregnant patientsCMV seronegative blood products should be provided to pregnancy women, regardless of CMV status.Components should also be provided for transfusions throughout pregnancy, for example in the case of haemoglobinopathies.HIV and immunodeficient patientsThese patients should receive leucodepleted blood as there is no evidence to suggest a benefit with the use of CMV seronegative componentsOrgan transplant patientsOrgan transplant patients should receive leucodepleted blood onlyCMV PCR should be used to assess CMV infection for patient groups to enable early detection and treatmentGranulocytesGranulocyte components provided should be CMV seronegative for all patients as these components cannot be leucodepleted6.5Potential impact on blood centre employees includes the reduction in workload. Considerations needs to be given towards how this workload can be replaced. Consideration also needs to be given towards the disaster of redundancy, as a successive effect of this proposal.6.6The board must be aware of the clinical and monetary benefits of this proposal however, the board should also be aware of potential limitations regarding the operation of the proposal. The board should also be aware of potential legal repercussions should someone become infected with CMV through a blood component.6.7Stakeholders that will need to be involved include both internal and external. Internal stakeholders will include the manager of the NHSBT site and the head of testing. External stake holders will need to raise public sensation regarding the change in production of seronegative CMV components. Doctors will also need to be aware of the changes implemented to CMV negative components and be aware of who this applies for. E.g. certain patient groups will still receive CMV seronegative components.ReferencesA. Ross, S., Novak, Z., Pati, S. and B. Boppana, S. (2011). Overview of the Diagnosis of cytomegalovirus transmitting. Infectious Disorders Drug Targets, 11(5), pp.466-474.Azevedo, L., Pierrotti, L., Abdala, E., Costa, S., Strabelli, T., Campos, S., Ramos, J., Latif, A., Litvinov, N., Maluf, N., Caiaffa Filho, H., Pannuti, C., Lopes, M., Santos, V., Linardi, C., Yasuda, M. and Marques, H. (2015). Cytomegalovirus infection in transplant recipients. Clinics, 70(7), pp.515-523.Crough, T. and Khanna, R. (2009). Immunobiology of Human Cytomegalovirus from Bench to Bedside. Clinical Microbiology Reviews, 22(1), pp.76-98.DOH UK, (2012). SaBTO Report of Cytomegalovirus Tested Blood Components, Position Statement. online pp.1 15. Available at https//www.gov.uk/government/uploads/system/uploads/attachment_data/file/215125/dh_133086.pdf Accessed 13 Mar. 2017.Drew, W. and Roback, J. (2007). Prevention of transfusion-transmitted cytomegalovirus reactivation of the debate? Transfusion, 47(11), pp.1955-1958.Guidelines for the Blood Transfusion S ervices in the United Kingdom. 8th Edition, TSO Norwich, http//www.transfusionguidelines.org/transfusion-handbook/3-providing-safe-blood. Accessed 25/10/2016Kumar, H., Gupta, P., Mishra, D., Sarkar, R. and Jaiprakash, M. (2006). Leucodepletion and Blood Products. Medical Journal Armed Forces India, 62(2), pp.174-177.Ljungman, P. (2004). luck of cytomegalovirus transmission by blood products to immunocompromised patients and means for reduction. British Journal of Haematology, 125(2), pp.107-116.Pang, X., Fox, J., Fenton, J., Miller, G., Caliendo, A. and Preiksaitis, J. (2009). Interlaboratory Comparison of Cytomegalovirus Viral Load Assays. American Journal of Transplantation, 9(2), pp.258-268.Pennington, J., Garner, S., Sutherland, J. and Williamson, L. (2001). Residual subset population analysis in WBC-reduced blood components using real-time PCR quantitation of specific mRNA. Transfusion, 41(12), pp.1591-1600.Roback, J. (2002). CMV and blood transfusions. Reviews in Medical Virol ogy, 12(4), pp.211-219.Roback, J., Drew, W., Laycock, M., Todd, D., Hillyer, C. and Busch, M. (2003). CMV DNA is rarely detected in healthy blood donors using validated PCR assays. Transfusion, 43(3), pp.314-321.Roback, J., Hillyer, C., Drew, W., Laycock, M., Luka, J., Mocarski, E., Slobedman, B., Smith, J., Soderberg-Naucler, C., Todd, D., Woxenius, S. and Busch, M. (2001). Multicenter evaluation of PCR methods fordetecting CMV DNA in blood donors. Transfusion, 41(10), pp.1249-1257.Seed, C., Wong, J., Polizzotto, M., Faddy, H., Keller, A. and Pink, J. (2015). The residual risk of transfusion-transmitted cytomegalovirus infection associated with leucodepleted blood components. Vox Sanguinis, 109(1), pp.11-17.Sia, I. and Patel, R. (2000). New Strategies for Prevention and Therapy of Cytomegalovirus Infection and Disease in Solid-Organ Transplant Recipients. Clinical Microbiology Reviews, 13(1), pp.83-121.Wolff, D., Heaney, D., Neuwald, P., Stellrecht, K. and Press, R. (2009). Multi- Site PCR-Based CMV Viral Load Assessment-Assays Demonstrate Linearity and Precision, but Lack Numeric Standardization. The Journal of Molecular Diagnostics, 11(2), pp.87-92.Ziemann, M. and Hennig, H. (2014). Prevention of Transfusion-Transmitted Cytomegalovirus Infections Which is the Optimal Strategy?. Transfusion care for and Hemotherapy, 41(1), pp.7-7.Ziemann, M., Unmack, A., Steppat, D., Juhl, D., Grg, S. and Hennig, H. (2010). The natural course of primary cytomegalovirus infection in blood donors. Vox Sanguinis, 99(1), pp.24-33.
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