Study design

The collection and use of human-subject materials was approved by the Ethical Committee on Human Subjects of each participating institute. We obtained informed consent from the parents of all enrolled newborns. The screening method and study outline are illustrated in figure 1. The National Institute for Infectious Diseases (NIID) in Tokyo distributed filters with ID numbers to all study sites. The ID numbers consisted of five digit numbers, indicating <area>-<study site within the area>-<three digits for each newborn ID at the site>. We collected urine on a 2 cm×5 cm piece of FTA-Elute filter cards (Whatman) inserted into the diaper of each newborn within 4 days of birth and before discharge. After removal from the diaper, the urine filter was dried and mailed to NIID, where it was received within 1–2 days of shipment. The qPCR described in the following section was performed shortly after receipt of the specimens (mean of 1.1±1.2 days). Approximately 70% of distributed filter cards were recovered for screening. The main reasons for the non-return of filters were (1) that they were used to demonstrate urine collection techniques to the nurses and paramedicals; (2) repeated urine collection owing to insufficient urination prior to diaper change; (3) too much stool on the filter; and (4) misplacement of the initial filter. All filters were accounted for as the NIID sent each study site an Excel file containing information regarding filter ID, date of receipt of the specimens, and test results after each qPCR run, and each study site added the results to the newborns' medical records. There were about 20 occasions on which the study sites emailed or called NIID because of a typographical error in the filter ID in the file.

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Figure 1

Screening method and study design. ABR, auditory brainstem responses; CMV, cytomegalovirus; DBS, dried blood spot; GCV, ganciclovir; VGCV, valganciclovir.

When the test result was positive, physicians contacted the parents to arrange an immediate clinic visit for the collection of urine and blood specimens from the newborns to confirm congenital CMV infection. Specimens for confirmation were collected at the age of 15.8±3.8 days (range 7–21 days). Virus isolation, virus load measurement and serology were performed using these specimens. In addition to urine specimens, dried umbilical cord specimens were obtained from 23 of the cases for further confirmation.

We obtained separate informed consent to use DBS specimens from the cases retrospectively for our study, and requested the incorporated foundations handling DBSs for sending the specimens. DBS specimens were retrieved from 12 of the cases, 11 of which were asymptomatic, and one had SNHL at birth. Blood specimens were obtained from mothers and urine specimens from siblings.

We established 25 study sites in six geographically separate areas of Japan. The study sites serve rural, rural–urban, and urban/metro societies. More than 99.9% of all babies born at the sites were recruited for enrolment, and 1.3% of their parents refused participation. A few infants severely ill in neonatal intensive care units (NICUs) were excluded owing to difficulties in the collection of urine. Enrolment was carried out from April 2008 to September 2010. The sites included primary obstetric clinics and municipal hospitals (type 1 sites), as well as university-associated and national hospitals (type 2 sites) that care for the general population of pregnant women as well as patients referred from type 1 clinics. Pregnant women are able to select clinics/hospitals according to their preference. Type 2 sites are generally large in scale, have a NICU and employ specialists in most clinical areas. Type 1 sites include Mori Hospital, Tomakomai City Hospital, Sapporo Tokusyukai Hospital, Nihonmatsu Hospital, Yamaguchi Hospital, Toyokawa City Hospital, Wakamiya Hospital, Palmore Hospital, Hanamizuki Ladies Clinic, Fujita Clinic, Fuchi Ladies Clinic, Miura Clinic for Women and Children, Miyamura Hospital and Takara Maternity Clinic. Type 2 sites include National Fukushima Hospital, National Centre for Child Health and Development, Iwaki Kyoritsu Hospital, Hyogo Prefectural Kobe Children's Hospital and Kariya Toyota General Hospital, and hospitals at Asahikawa Medical University, Fukushima Medical University, Tokyo University, Fujita Health University, Kobe University and Nagasaki University.

qPCR for screening

We punched a 3 mm diameter disc from the urine filters, washed this with 200 μl of water and then transferred it into 50 μl of qPCR reaction mixture in a well of a 96-well plate. Only one filter disc can be submerged into the reaction mixture after brief centrifugation (400 g, 30 s). The qPCR assay for the CMV UL84 fragment and thermal cycling conditions were described previously.2 15 Although it is ideal to include an internal control to ensure the absence of PCR inhibition, we did not do so in this study for the following reasons: (1) although we initially spiked irrelevant DNA/primers/probe into the qPCR reaction mixture for screening (n=200 urine-filters) to check the efficiency of qPCR, no cases of inhibition were observed; (2) our previous study15 demonstrated a close correlation in viral load measurements between the urine-filter-based qPCR assay and the common qPCR assay using DNA samples purified from liquid urine; and (3) to reduce cost as far as possible. To confirm positive results in the screening qPCR, DNA samples were recovered from four 3 mm diameter filter discs by incubation at 95°C for 30 min in 50 μl of water containing 100 ng of carrier DNA, and 5 μl aliquots of the recovered DNA samples were used for qPCR.15 Simple mathematical consideration of the detection efficiencies (15–20% in qPCR containing urine-filter vs 60% in qPCR using eluted DNA samples) and the number of used filter discs indicates that both qPCR assays detect almost equivalent amounts of CMV DNA. The cost for our test itself, including the filter paper, reagents, disposables and technical labour for the assay, was <750 Yen (∼£5.50, €7 or US$9) per study participant.

DNA preparation from specimens other than urine filters

DNA samples were purified from liquid urine using a Viral RNA kit (Qiagen, Hilden, Germany), and from whole blood using a QIAamp DNAmini kit (Qiagen) according to the manufacturer's instructions. DNA was purified from dried umbilical cord2 and DBS8 specimens as described previously. The efficiency of DNA recovery from DBS specimens was >90%.11

Clinical and audiological evaluation

Clinical data for newborns, including birth weight, gestational age (GA), clinical manifestations and abnormal laboratory findings, were extracted from their medical records. The mental and physical development of infected infants has been closely monitored at outpatient clinics. Audiological testing was carried out using auditory brainstem responses and/or auditory steady-state responses, and brain imaging was carried out by CT and/or magnetic resonance images. Although interpretation of mild abnormalities in brain images is sometimes difficult, our Study Group contains a specialist with long experience in paediatric neurology and brain imaging. Medical records of mothers were examined for abnormalities during pregnancy. We defined ‘typical clinical manifestations’ as any of microcephaly, chorioretinitis, SNHL or a combination of petechiae, hepatosplenomegaly and jaundice. Intrauterine growth restriction (IUGR) and any single, mild manifestation were discounted as ‘typical clinical manifestations.’ ‘Symptomatic’ cases were defined as those exhibiting any typical clinical manifestations and/or abnormalities in their brain images.

Prior to the initiation of screening, our Study Group prepared a tentative guideline for antiviral treatment based on the same protocol and inclusion/exclusion criteria used in the published clinical trial.16 Treatment was performed based on the criteria and informed consent.

Strain analysis and serology

Sequences of the polymorphic regions of the gN, UL144, and UL146 genes of CMV strains were determined as described previously.17 18 In contrast to European countries, only 10% of obstetric clinics/hospitals in Japan conduct routine CMV serology for pregnant women. In this study, two study sites performed a CMV-specific IgG test for all pregnant mothers (n=4877), and some sites tested CMV-IgG of pregnant women with any risk factors (n=524) at 10–20 weeks of pregnancy. Each of those sites used one of the following additional tests; CMV-IgG avidity test for seropositives at 19 weeks of pregnancy, CMV-IgG test for seronegatives at 35–36 weeks of pregnancy, and CMV-IgG and -IgM tests for seronegatives during the middle and late terms of pregnancy. All of their babies except for refusals were enrolled for CMV screening after birth. Serology tests for CMV-specific IgG and IgM were carried out at a commercial laboratory (SRL, Tokyo, Japan) using EIA kits produced at DENKA SEIKEN Co. (Niigata, Japan). The CMV-IgM kit is based on the IgM-captured sandwich method using CMV-specific antibodies for detection. The CMV-IgG avidity test was carried out at Aisenkai Nichinan Hospital as described previously.19

Statistical methods

Statistical significance was evaluated using the χ² test. The Mann–Whitney U test was used to analyse differences in virus loads between two groups. We used a website (http://www.measuringusability.com/wald.htm) to calculate adjusted Wald 95% CIs.