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Hong, Kim, Park, Jung, Lee, Chong, Sung, Lee, Choi, Kim, Woo, and Kim: Sensitivity of the Cytomegalovirus Antigenemia Assay to Diagnose Cytomegalovirus Retinitis
Original Article

Infection & Chemotherapy 2016; 48(4): 302-308.

Published online: 22 November 2016

DOI: https://doi.org/10.3947/ic.2016.48.4.302

Sensitivity of the Cytomegalovirus Antigenemia Assay to Diagnose Cytomegalovirus Retinitis

Sun In Hong1, 2, Taeeun Kim2, Se Yoon Park3, Jiwon Jung4, Joo Yong Lee5, Yong Phil Chong2, Heungsup Sung6, Sang-Oh Lee2, Sang-Ho Choi2, Yang Soo Kim2, Jun Hee Woo2, Sung-Han Kim2

1Department of Infectious Diseases, Gyeongsang National University Changwon Hospital, Gyeongsang National University School of Medicine, Changwon, Korea.

2Department of Infectious Diseases, Asan Medical Center, University of Ulsan College of Medicine, Seoul, Korea.

3Division of Infectious Diseases, Department of Internal Medicine, Soonchunhyang University Seoul Hospital, Soonchunhyang University College of Medicine, Seoul, Korea.

4Division of Infectious Diseases, Department of Internal Medicine, Ulsan University Hospital, University of Ulsan College of Medicine, Ulsan, Korea.

5Department of Ophthalmology, Asan Medical Center, University of Ulsan College of Medicine, Seoul, Korea.

6Department of Laboratory Medicine, Asan Medical Center, University of Ulsan College of Medicine, Seoul, Korea.

Corresponding author: Sung-Han Kim, MD. Department of Infectious Diseases, Asan Medical Center, University of Ulsan College of Medicine, 86 Asanbyeongwon-Gil, Songpa-Gu, Seoul 05505, Korea. Tel: +82-2-3010-3305, Fax: +82-2-3010-6970, kimsunghanmd@hotmail.com

Received 29 May 2016       Accepted 2 September 2016

Copyright © 2016 by The Korean Society of Infectious Diseases and Korean Society for Chemotherapy

(open-access, http://creativecommons.org/licenses/by-nc/3.0/):

This is an Open Access article distributed under the terms of the Creative Commons Attribution Non-Commercial License (http://creativecommons.org/licenses/by-nc/3.0/) which permits unrestricted non-commercial use, distribution, and reproduction in any medium, provided the original work is properly cited.

Abstract

Background

Cytomegalovirus (CMV) retinitis is one of the most important tissue-invasive CMV diseases in immunocompromised patients. Since 1980, non-invasive diagnostic methods, notably the CMV antigenemia assay, have been widely used as adjunct tests to diagnose tissue-invasive CMV diseases. However, there are limited data on the diagnostic value of the CMV antigenemia assay for diagnosing CMV retinitis.

Materials and Methods

We performed a retrospective review of all cases of CMV retinitis at Asan Medical Center, Seoul, South Korea over a 9-year period. The diagnosis of CMV retinitis was made by experienced ophthalmologists according to medical history and an ophthalmoscopic appearance of typical retinopathy, together with absence of an alternative diagnosis.

Results

We analyzed 44 patients with CMV retinitis (affecting 57 eyes) for whom the CMV antigenemia assay was performed. Of the 44 patients, 31 (70%) were HIV-uninfected and 13 (30%) were HIV-infected. The overall sensitivity of the CMV antigenemia assay was 66% (95% confidence interval [CI] 50–80%). The test’s sensitivity showed a non-significant trend towards being higher in HIV-infected patients than in HIV-uninfected patients (sensitivity 85% vs 58%, respectively, P = 0.16). In a subgroup analysis of the 35 patients without other concurrent tissue-invasive CMV disease, the sensitivity of the CMV antigenemia assay was 57% (95% CI 40–74%).

Conclusions

The CMV antigenemia assay has limited value as a non-invasive diagnostic adjunct test for CMV retinitis. Therefore, the results of the assay need to be interpreted in the context of underlying disease, clinical presentation, and ophthalmoscopic findings.

Keywords: Cytomegalovirus, Retinitis, Diagnosis, Test

Introduction

Cytomegalovirus (CMV) disease is an important cause of morbidity and mortality among patients with impaired cellular immunity, including patients who have received solid organ transplants (SOT) or hematopoietic stem cell transplants (HCT), are undergoing chemotherapy for malignant disease, or are HIV-infected [1]. Of the various end organ diseases of CMV infection, CMV retinitis is the most common, and is the leading cause of disability in HIV-infected patients [2]. In addition, since the numbers of patients with SOT, HCT, and malignancy undergoing chemotherapy are increasing, the incidence of CMV retinitis is expected to increase [3]. Hence, accurate diagnosis and treatment of CMV retinitis is important in HIV-uninfected immunocompromised patients as well as in HIV-infected patients.
CMV retinitis is diagnosed by experienced ophthalmologists based on the patient’s medical history, an ophthalmoscopic appearance typical of CMV retinopathy, and laboratory assessment of immune status that eliminates HIV retinopathy, toxoplasma retinitis, acute retinal necrosis, progressive outer retinal necrosis, and syphilitic retinochoroiditis [4]. The characteristic appearance of the infection is sufficiently distinctive that other diagnostic procedures are rarely needed. However, atypical cases, or infections with other organisms in patients at high risk of CMV retinitis, may require invasive diagnostic tests such as vitreous sampling. Furthermore, even invasive diagnostic tests may fail to establish the diagnosis. Since 1980, non-invasive diagnostic methods, such as the CMV antigenemia assay, have been widely used as adjunct tests for the diagnosis of tissue-invasive CMV diseases. However, data on the diagnostic value of the CMV antigenemia assay for CMV retinitis are limited [5]. Therefore, to assess its value, we compared the sensitivity of the CMV antigenemia assay to diagnose CMV retinitis in HIV-infected and HIV-uninfected patients.

Materials and Methods

1. Patient selection and method of CMV antigenemia assay

We reviewed the medical records of patients diagnosed with CMV retinitis between January 2005 and December 2013 in a 2,700-bed tertiary-care hospital in Seoul, Korea, where the prevalence of HIV infection is low. The CMV antigenemia assays used were the Light Diagnostics CMV pp65 antigenemia assay (Millipore Corp., Temecula, CA, USA), used from January 2005 to February 2012, and the CINAkit Rapid Antigenemia assay (Argene, North Massapequa, NY, USA), used from March 2012 to December 2013. These were performed as previously described [6]. Briefly, about 5 mL of blood was mixed with 1.5 mL of 6% dextran in saline and allowed to sediment. The polymorphonuclear leukocyte-enriched supernatant was extracted. Contaminating erythrocytes were lysed with a 0.8 NH4Cl solution. After two washing steps, leukocyte suspensions were counted and adjusted to 1 × 106 cells/mL. A total of approximately 2 × 105 cells were spotted on a slide by cytocentrifugation, fixed in a 5% formaldehyde solution, and stained by immunofluorescent assay using a monoclonal antibody directed against the pp65 CMV antigen [7]. Counts were expressed as positive cells per 2 × 105 leukocytes [89].
In kidney transplantation recipients, repeated CMV antigenemia assays were performed to monitor CMV infection at 1, 2, 3, 4, 6, 8, 12, 16, 20, and 24 weeks after transplantation [10]. In patients who underwent HCT, CMV antigenemia assays were performed weekly from day 21 to day 100 post-HCT, then monthly until one year after HCT [11]. Surveillance testing using the CMV antigenemia assay in patients with other underlying diseases was performed at the discretion of the attending physician.

2. Definition of CMV retinitis and outcomes

CMV retinitis was defined as presence of the characteristic ophthalmoscopic picture of necrotizing retinitis with or without hemorrhage, as determined by an ophthalmologist [4]. The diagnosis of CMV retinitis was confirmed by review of fundoscopic findings by an experienced retinal specialist JY Lee.
Best corrected visual acuity (BCVA) was measured using Snellen charts. BCVA was assessed whenever patients visited the ophthalmologist. Stable vision was defined as either the maintenance or improvement of BCVA subsequent to receiving a diagnosis of CMV retinitis. Worsening vision was defined as BCVA declining by ≥1 line. Visual loss was defined as a complete lack of light perception. “Default” was defined as being lost to follow-up because of death or transfer to another hospital. “Other” was defined when the result could not be analyzed because of the presence of other ophthalmologic diseases.

3. Literature Review

We searched PubMed (which contains citations over the 30 years from 1985 to September 2014) for English-language literature on HIV-uninfected patients aged older than19 years with CMV retinitis. We used the search terms "cytomegalovirus", "retinitis", "NOT acquired immunodeficiency syndrome", and "NOT HIV". A total of 196 articles were found; 12 included the results of the CMV antigenemia assays. In addition, we searched the Korean-language literature in KoreaMed in a similar manner.

4. Statistical analysis

All statistical analyses were performed using SPSS version 21.0 (SPSS, Chicago, IL, USA). Categorical variables were compared using Fisher’s exact test or Pearson chi-square test, as appropriate. Continuous variables were compared using the Mann-Whitney U-test or Student’s t-test. All tests were two-tailed and differences were considered significant at P <0.05.

5. Ethics statement

The study was approved by the Institutional Review Board of Asan Medical Center (No. 2013-1040) and the requirement for informed consent was waived because of the retrospective nature of the study.

Results

Fifty-two patients with CMV retinitis were identified. Eight were excluded because they had no CMV antigenemia assay performed. Of the remaining 44 patients, 31 (70%) were HIV-uninfected. The cutoff value for a positive CMV antigenemia assay was set at one positive cell per 2 × 105 leukocytes. The results were positive in 29 (66%) of 44 patients and negative in the remaining 15 (34%) patients. The baseline clinical characteristics and outcomes of the patients with positive and negative CMV antigenemia results are presented in Table 1. The overall sensitivity of the CMV antigenemia assay was 66% (95% confidence interval [CI], 50–80%) (Table 2), showing a tendency to be higher in the HIV-infected patients (85% [11/13]) than in the HIV-uninfected patients (58% [18/31]), but this effect did not reach statistical significance (P = 0.16). Of the 31 HIV-uninfected patients, 10 had undergone SOT and 13 had undergone HCT. CMV retinitis was diagnosed at a median interval of 190 days (interquartile range [IQR] 140–430 days) and 84 days (IQR 44–233 days) post-transplantation in those who received SOT and HCT, respectively. Of these 23 patients, 5 (22%) had neutropenia (absolute neutrophil count ≤1.5 cells × 109/L) at the time they were diagnosed with CMV retinitis and 2 (9%) had severe neutropenia (absolute neutrophil count ≤0.5 cells × 109/L). The sensitivity of the CMV antigenemia assay in neutropenic patients was 40% (2/5) and in non-neutropenic patients was 61% (11/18). If patients with concurrent CMV diseases (n = 9) were excluded from the analysis, the sensitivity of the CMV antigenemia assay was 57% (20/35, 95% CI 40–74%) (Table 2). Twenty-seven of the 35 patients without concurrent CMV diseases were HIV-uninfected; the sensitivity of the assay in HIV-uninfected and HIV-infected patients was 52% (14/27) and 75% (6/8), respectively.
Table 1

Clinical characteristics and outcomes in patients with CMV retinitis who showed positive and negative CMV antigenemia result

ic-48-302-i001
Total (n = 44) CMV antigenemia positive (n = 29) CMV antigenemia negative (n = 15) P-value
Age, years, mean ± SD 46.1 ± 14.5 48.3 ± 13.5 41.9 ± 16.0 0.19
Bi-ocular involvement 13 (30) 10 (35) 3 (20) 0.49
Underlying disease:
 HCT 13 (30) 8 (28) 5 (33) 0.74
 Lymphoma 2 (5) 1 (3) 1 (7) >0.99
 Solid organ transplant 10 (23) 5 (17) 5 (33) 0.27
 HIV 13 (30) 11 (38) 2 (13) 0.09
 Solid tumora 3 (7) 2 (7) 1 (7) >0.99
 Otherb 3 (7) 2 (7) 1 (7) >0.99
Anti-CMV therapy:
 Systemic antiviral agents 22 (50) 13 (45) 9 (60) 0.34
 Combined systemic and intravitreal injection 19 (43) 15 (52) 4 (27) 0.11
 Intravitreal injection 2 (5) 0 2 (13) 0.11
 None of the above 1 (2) 1 (3) 0 >0.99
Other concurrent CMV disease:
 GI CMV disease 8 (18) 8 (28) 0 0.04
 CMV hepatitis 1 (2) 1 (3) 0 >0.99
Outcome:
 Stable 23 (52) 14 (48) 9 (60) 0.46
 Progression 8 (18) 6 (21) 2 (13) 0.55
 Visual loss 4 (9) 3 (10) 1 (7) >0.99
 Default 7 (16) 5 (17) 2 (13) >0.99
 Other 2 (5) 1 (3) 1 (7) >0.99
Data are presented as number (%), unless otherwise indicated.
aTwo patients had thymomas and one had a pancreatic cancer.
bOne patient without underlying disease was treated in the intensive care unit for one month because of complicated methicillin-sensitive Staphylococcus aureus bacteremia with multiple metastatic infections; another had dyskeratosiscongenita, and the third had interstitial lung disease; the latter two patients were treated with cyclosporine.
CMV, cytomegalovirus; SD, standard deviation; HCT, hematopoietic stem cell transplants; HIV, human immunodeficiency virus; GI, gastrointestinal.
Table 2

Comparison of the sensitivity of the CMV antigenemia assay in HIV-uninfected and HIV-infected patients with CMV retinitis

ic-48-302-i002
Total (n = 44) No concurrent CMV disease (n = 35)
HIV-uninfected (n = 31) HIV-infected (n = 13) P-value HIV-uninfected (n = 27) HIV-infected (n = 8) P-value
Positive CMV antigenemiaa (%) 18 (58) 11 (85) 0.16 14 (52) 6 (75) 0.42
Peak level of CMV antigenemia (range) 9 (0–46) 7 (7–30) 0.70 4 (0–38) 4 (0–12) 0.89
Data are presented as number (%) or median (interquartile range).
aOne or more positive cell per 200,000 leukocytes was considered a positive CMV antigenemia assay.
CMV, cytomegalovirus; HIV, human immunodeficiency virus
Overall, 23 (52%) patients had stable visual outcomes. Two of these underwent vitrectomy due to vitreous hemorrhage; their BCVAs improved. During the treatment of CMV retinitis, BCVA declined in 8 patients (17%) and 4 (9%) had no light perception. Three patients (7%) with CMV-related retinal detachment underwent retinal re-attachment surgery. The BCVA had deteriorated in 2 of these patients, and the remaining patient had no light perception. There were no statistically significant differences in outcomes between the HIV-infected and HIV-uninfected patients. The median follow-up duration of the 35 patients who did not default was 16.7 months (IQR 157–1,086 months).
We performed a literature review to determine the performance of the CMV antigenemia assay in CMV retinitis in HIV-uninfected patients (Table 3). CMV antigenemia assay results were available for a total of 18 patients among all the patients included in the 12 articles identified. The overall sensitivity of the CMV antigenemia assay in the literature review was 61% (11/18).
Table 3

Literature review of the results of the CMV antigenemia test in HIV-uninfected patients with CMV retinitis

ic-48-302-i003
UPN [ref] Sex / Age Value of CMV antigenemiaa Underlying disease Treatment
1 [12] F/20 negative ALL s/p unrelated BMT Foscarnet / intravitreal GCV
2 [13] b F/27 600 / 2 × 105 Lung transplantation Foscarnet
3 [14] M/58 66 / 5 × 104 NHL s/p ASCT GCV
4 [15] M/26 Negative azathioprine, prednisolone with CVI GCV
5 [16] M/42 Negative FK, MMF, prednisolone s/p KT GCV / intravitreal GCV
6 [16] M/31 Positive CsA, MZ, prednisolone s/p KT GCV
7 [16] M/50 Negative FK, MZ, prednisolone s/p KT GCV
8 [16] M/42 Negative FK, MMF, prednisolone s/p KT GCV
9 [17] F/51 >50 / 4 × 105 Immunocompetent GCV / intravitreal GCV
10 [18] F/51 Negative Prednisolone, azathioprine with DM GCV
11 [19] F/36 12 / 2 × 105 AML s/p BMT GCV
12 [20] M/38 10 / 1.5 × 105 ALL s/p BMT GCV
13 [20] F/43 6 / 1.5 × 105 NHL s/p BMT GCV
14 [20] F/57 28 / 1.5 × 105 AML s/p BMT GCV / intravitreal GCV
15 [20] F/41 4 / 1.5 × 105 ALL s/p BMT GCV
16 [21] F/57 2400 / 5 × 105 Cyclophosphamide, azathioprine, anti-TNF Ab with RA GCV
17 [22] F/61 9 / 2 × 104 Intravitreal bevacizumab injection with diabetes retinopathy GCV
18 [23] F/52 Negative Dexamethasone, cyclosporine with T-LGLL GCV / intravitreal GCV
19-27 [24] M (88%)/NA NA KT (1), SLE (1), lymphoma (3), AA (4) NA
28-42 [25] M (93%)/36 NA AIDS various
43-58 [26] M (81%)/33 NAc s/p BMT various
59-77 [27] M (63%)/14 NA various various
aData are number of positive cells per number of leukocytes.
bOnly UPN 2 had another concurrent CMV disease: CMV pneumonia.
cSix among 16 CMV retinitis patients (38%) showed positive results in either CMV antigenemia assay or CMV PCR.
UPN, unique patient number; CMV, cytomegalovirus; ALL, acute lymphoblastic leukemia; BMT, bone marrow transplantation; GCV, ganciclovir; NHL, non-Hodgkin's lymphoma; ASCT, autologous; stem cell transplantation; CVI, common variable immunodeficiency; FK, tacrolimus; MMF, mycophenolate mofetil; KT, kidney transplant; CsA, cyclosporine A; MZ, mizoribine; DM, dermatomyositis; AML, acute myeloid leukemia; TNF, tumor necrosis factors; RA, rheumatoid arthritis, T-LGLL, T cell large granular lymphocytic leukemia; s/p, status post; SLE, systemic lupus erythematosus; AA, aplastic anemia; AIDS, acquired immunodeficiency syndrome; NA, not applicable

Discussion

The CMV antigenemia assay has been used to detect CMV reactivation in a variety of clinical settings [528]. It has the advantages of providing results within 24 hours and being quantifiable. Its introduction has considerably improved the clinical management of CMV disease in allogeneic HCT and SOT recipients, using a preemptive approach. However, studies of the diagnostic value of the CMV antigenemia assay in CMV retinitis are limited. We previously showed that the CMV antigenemia test was positive in 54% (26/57; 95% CI 41–68%) of patients with CMV gastrointestinal disease and 69% (25/36; 95% CI 52–84%) of patients with CMV pneumonia, suggesting that it has low sensitivity for ruling out these 2 conditions [89]. Xharrd et al. [3] reported that the CMV antigenemia test or CMV PCR were negative in all of 6 hematopoietic stem cell transplant patients with CMV retinitis. Eid et al. [29] also found that only 4 of 9 (44%; 95% CI 18–74%) solid organ transplant recipients with CMV retinitis tested positive for CMV PCR or CMV culture. In the present study, the test’s sensitivity in HIV-uninfected patients was 58% (18/31; 95% CI 42–74%). If patients with other concurrent CMV infections were excluded from the analysis, the sensitivity was 52% (14/27; 95% CI 33–70%), suggesting that the assay is not useful for ruling out CMV retinitis. Interestingly, there was a statistically non-significant trend for the sensitivity in HIV-uninfected patients to be lower (58%) than in HIV infected patients (85%, P = 0.16). Such variable sensitivity might possibly reflect differences in the causes of CMV retinitis in HIV-uninfected patients compared with HIV-infected patients. Further studies are needed in this area.
Our study had several limitations. First, by virtue of its retrospective design, we could not gather clinical data at the time of presentation in all of the patients. Furthermore, because the patient population was heterogeneous, follow-up was not standardized. Second, due to the specific circumstances of the Korean national medical insurance system, CMV PCR was not routinely performed for surveillance. The CMV antigenemia assay does not require expensive equipment and the associated costs are low. But it is time-consuming, labor-intensive, and requires a high level of technical expertise. In addition, there is no assay standardization and poor inter-institutional correlation exists. False negative results for CMV antigenemia can occur in patients with leukopenia [28303132]. Furthermore, CMV antigenemia has a lower sensitivity than CMV PCR. However, in the light of previous results, it can be assumed that the use of PCR would not have yielded very different results [11]. Third, because patients who did not have CMV antigenemia assay results were excluded from the study population, there may have been some selection bias. Lastly, CMV retinitis is a rare disease. Therefore, the study patients were collected over a 9-year period. The medical management of patients after transplantation or on immunosuppressive therapy clearly changed over this period.
In conclusion, the CMV antigenemia assay has limited value as a noninvasive diagnostic adjunct test for CMV retinitis. Because of the high cost of a false-negative diagnosis of CMV retinitis the results of the assay need to be interpreted in the context of the underlying disease, clinical presentation, and ophthalmoscopic findings.

Notes

This paper was presented in part at the 55th Interscience Conference on Antimicrobial Agents and Chemotherapy, San Diego, 17-21 September 2015 (Poster session, abstract no. T-1367).

This work was supported by a grant from the Korea Health Technology R&D Project through the Korea Health Industry Development Institute (KHIDI), funded by the Ministry of Health & Welfare, Republic of Korea (grant no. HI15C1763).

Conflict of Interest No conflicts of interest.

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TOOLS
ORCID iDs

Sun In Hong
https://orcid.org/http://orcid.org/0000-0003-2575-2084

Taeeun Kim
https://orcid.org/http://orcid.org/0000-0002-2075-4497

Se Yoon Park
https://orcid.org/http://orcid.org/0000-0002-4538-7371

Jiwon Jung
https://orcid.org/http://orcid.org/0000-0003-4333-3270

Sung-Han Kim
https://orcid.org/http://orcid.org/0000-0002-6596-8253

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