Clinical and Diagnostic Laboratory Immunology, September 1998, p. 632-635, Vol. 5, No. 5
1071-412X/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.
Age-Related Changes in Blood Lymphocyte Subsets of
Saudi Arabian Healthy Children
S.
Shahabuddin,1,*
I.
Al-Ayed,2
M. O. Gad
El-Rab,1 and
M.
I.
Qureshi2
Division of Immunology, Department of
Pathology,1 and
Department of
Pediatrics,2 College of Medicine and King
Khalid University Hospital, King Saud University, Riyadh 11461, Kingdom
of Saudi Arabia
Received 16 January 1998/Returned for modification 10 March
1998/Accepted 26 May 1998
 |
ABSTRACT |
The age-related changes in absolute and percentage values of
lymphocyte subsets in the peripheral blood of healthy children of
different ages (1 month to 13 years) were studied by flow cytometry. The absolute and percentage values for most lymphocyte subpopulations differed substantially with age. Comparisons among age groups from
infants through adults revealed progressive declines in the absolute
numbers of leukocytes, total lymphocytes, and T, B, and natural killer
(NK) cells. The percentages of T cells increased with age. Within the
T-lymphocyte population, the CD8+ subset increased but the
CD4+ subset decreased, resulting in a declining
CD4+/CD8+ ratio. The percentage of B cells
declined, but that of NK cells remained unchanged. The percentage of
HLA-DR+ T cells increased over time, but their number
changed inconsistently. Our findings confirm and extend earlier reports
on age-related changes in lymphocyte subpopulations. These data should
be useful in the interpretation of disease-related changes, as well as
therapy-dependent alterations, in lymphocyte subsets in children of
different age groups.
| |
INTRODUCTION |
Immunophenotyping of blood
lymphocytes, or lymphocyte subset analysis, with monoclonal antibodies
by flow cytometry is used routinely in the diagnosis of congenital and
acquired immune deficiency syndromes, as well as leukemia and lymphoma,
in children. In order to make a precise evaluation of affected
individuals, reference values for lymphocyte subpopulations during
childhood must be determined.
Age-related changes in blood lymphocyte subpopulations among healthy
children have been reported, but their values are not yet well
established for different age groups. Some studies on the reference
ranges for T and B lymphocytes and their subsets in infants and
children were done, but only a few lymphocyte markers were used
(1, 4, 6, 15). Most of these earlier studies of age-related
lymphocyte changes have been restricted to newborns (2, 7, 8, 13,
18, 24, 26, 31) or very young children (3) or have
compared young adults to older adults (16, 21). Few reports
have systemically documented immunophenotypic changes from birth
through adulthood (5, 9-12, 17, 19, 30, 33, 34).
In the present study, age-related values for healthy infants and
children of T, B, and natural killer (NK) cells and T-cell subsets in
peripheral blood were determined and compared with corresponding values
for healthy adults studied by the same technique.
| |
MATERIALS AND METHODS |
Subjects.
One hundred and two healthy children, 52 males and
50 females, with ages ranging from 1 month to 13 years and 30 healthy
adult blood donors with ages ranging from 18 to 44 years were studied. All subjects were of Saudi Arabian origin. Informed consent from adult
blood donors and from a parent or guardian of every child was obtained.
The children had come to the healthy child clinic of King Khalid
University Hospital, Riyadh, Saudi Arabia, for a routine health checkup
or a vaccination. All children and adults were considered healthy if
they had no past history of any disease; had normal blood pressure,
pulse rate, and hemoglobin count; had no fever, cough, or infection;
were not on any medication; and (for the donors) had not donated blood
in the past 3 months. In addition, all children and adult blood donors
were screened for syphilis, human immunodeficiency virus, hepatitis B
virus, and hepatitis C virus infection by routine serologic tests and
were found negative. Blood samples were collected in EDTA tubes and used within 2 h of storage at room temperature. A complete blood count, including automated differential, was performed with a Coulter
Counter.
Subjects were grouped into five age categories: group 1, ages 1 through
11 months; group 2, ages 1 through 2 years; group 3, ages 3 through 5 years; group 4, ages 6 through 13 years; group 5, ages 18 through 44 years.
Flow cytometric analysis of lymphocyte subpopulations.
Whole-blood samples were stained with the Simultest immune monitoring
kit having dual-color monoclonal antibodies (Becton Dickinson, Mountain
View, Calif.) (Table 1). All samples were analyzed by a FACScan flow cytometer (Becton Dickinson) calibrated with
CaliBRITE beads and AutoCOMP software; immunophenotyping results were
obtained with SimulSET software (Becton Dickinson), as instructed by
the manufacturer. Briefly, 100-µl volumes of Simultest reagent were
added to separate tubes and incubated for 15 to 20 min. Lysing solution
(2 ml; Becton Dickinson) was added to each tube. Following 10 min of
incubation, the tubes were centrifuged to remove lysed red cells and
the cells were washed twice with the cell wash (Becton Dickinson).
Washed cells were resuspended in 0.5 ml of the cell wash and analyzed
immediately by the flow cytometer. Absolute lymphocyte subset counts
were obtained as the product of the absolute lymphocyte count derived
from a hematology analyzer and the percentages of the lymphocyte subset
populations of interest, derived from the flow cytometer.
Lymphocyte subset identification.
T cells were defined as
those cells expressing the CD3 antigen, and B cells were defined as
those cells expressing CD19. NK cells were identified by the presence
of CD16, CD56, or both and by the absence of the coexpression of CD3.
In most cases, the sum of lymphocyte lineage percentages (percent T
cells + percent B cells + percent NK cells) was 100% ± 4%
in each age group. This calculation works as a quality control
verification for all lymphocyte subset determinations by flow cytometry
and rules out the presence of any preparation artifacts in the samples.
CD4+ and CD8+ cells were defined by the
presence of CD4 and CD8, respectively, with coexpression of CD3.
Activated T cells were those cells expressing HLA-DR on
CD3+ T cells.
Statistical analysis.
Analysis of variance was conducted by
using the Statpac Gold statistical analysis package, version 3.2 (Walonick Associated, Inc., Minneapolis, Minn.). The results are
presented as the means ± 1 standard deviation of the percentage
and absolute number for each lymphocyte population. The statistical
significance of the observed differences in the percentages and numbers
of lymphocyte subsets for any two groups was evaluated by Student's
t test. A P value of <0.05 (two tailed) was
considered statistically significant.
| |
RESULTS |
Absolute counts of WBC and lymphocyte subpopulations.
The mean
of the absolute leukocyte (WBC) count declines sharply across age
groups by a factor of approximately 1.4, from 10,330 cells/mm3 in infants to 7,221 cells/mm3 in
older children (Table 2). The absolute
count for other cell types declines even more steeply: more than
twofold (from 6,918 to 2,782 cells/mm3) for total
lymphocytes, twofold (from 4,479 to 1,997 cells/mm3) for T
cells, fourfold (from 1,652 to 427 cells/mm3) for B cells,
and twofold (from 552 to 289 cells/mm3) for NK cells. In
all the cases, the decline is statistically significant
(P < 0.05). In comparison with those for the older children, the absolute counts of the total lymphocytes and T and B
cells for adults are even lower, while the absolute counts of WBC and
NK cells are higher; however, these differences are not statistically
significant (P > 0.05). Although, the decline is progressive over the five age groups studied, the decrease in lymphocyte subset counts from group 3 to group 4 is not statistically significant; but that from group 1 to group 2 is significant. The mean
values for lymphocytes and most of their subsets for group 2 and group
3 show significant decreases from those for group 1 and groups 1 and 2, respectively (P < 0.05).
Percentages of lymphocyte subpopulations.
The percentage of
lymphocytes in the total WBC population declines with age from 67.4%
of the WBC in infants (group 1) to 47.5% in young children (group 3)
to 38.2% in older children (group 4) and to 29.9% in adults (group 5)
(Table 3) (P < 0.05).
The absolute number of B cells drops more than twofold between group 1 and group 3, whereas the percentage of B cells declines less than
twofold over a longer time. This is because the rate of decline in
B-cell absolute numbers is steeper than the change in total lymphocytes. The percentage value drops from 23.8% in infants (groups
1 and 2) to 19.6% in group 3 children to 13.4% in group 4 children
and remains at 13.9% in adults (group 5) (P < 0.05 for the transition between infants and groups 3, 4, and 5 and between
group 3 and groups 4 and 5). T cells decline in number less rapidly
than total lymphocytes. Sixty-five percent of lymphocytes in infants
are T cells, but this increases to 73.3% in older children (P < 0.05) and to 74.3% in adults (P < 0.05).
There is no significant change in the percentage of NK cells from group
1 to group 4, because the decline of the absolute values of NK cells is
similar to that of the total lymphocyte count. However, the percentage
of NK cells for adults (14.2%) is significantly different from the
percentages of NK cells for groups 1 through 4 (P < 0.05). The percentage of NK cells varied from 8.1% for infants to
10.5% for older children.
T-cell subsets and activated T cells.
The analysis of the
age-related changes in the percentages and numbers of CD4+
and CD8+ lymphocytes per cubic millimeter and in the ratio
between these two major T-cell subsets (Table 3) indicates that in the
early stages of life, T lymphocytes with the helper/inducer phenotype prevail over the T cells with the suppressor/cytotoxic phenotype. A
progressive reduction in the percentages and numbers of
CD4+ lymphocytes develops in the second year of life
(P < 0.05 for the transition between group 1 and group
2). In contrast, an increase in the percentages of CD8+
lymphocytes has been observed (P < 0.05), while the
numbers of these cells per cubic millimeter decline from infancy up to
the age of 5 years, but later on do not vary greatly from the values for the group of adult donors. On the basis of the variations in the
values of CD4+ and CD8+ lymphocytes, the
CD4+/CD8+ ratio decreases from 2.1 for 1- to
11-month-old infants to 1.2 for 6- to 13-year-old children
(P < 0.05), while no further significant decrease was
observed in the values for the adult group.
The percentage of T cells expressing the activation marker HLA-DR
increases from 3.9% in group 1 to 6.3% in group 2 to 10.9% in group
4 to 10.4% in group 5. The transition between group 1 and other groups
is statistically significant (P < 0.05). The absolute
values of these cell populations vary from 276 to 235 cells/mm3, and the difference is not statistically
significant (P > 0.05).
| |
DISCUSSION |
The present findings show that the absolute and percentage values
for most lymphocyte markers differ substantially not only between
children and adults but also between children from different age
groups. Therefore, the reference values for lymphocyte subsets of
neither adults nor children of mixed-age groups can be used for infants
and children.
There is a significant decline from infants to adults in absolute
counts of WBC, total lymphocytes, T, B, and NK cells, and CD4+ and CD8+ T-cell subsets. These
observations confirm the findings of other investigations (9, 12,
30, 33, 34).
It has been known for nearly 60 years (14) that total WBC
and absolute lymphocyte counts are highest at birth and decline with
age. Although the absolute counts decline, the relative proportions of
lymphocyte subsets vary, and total T-cell and CD8+ T-cell
percentages increase with age (4). Two more-recent studies
have reported that the percentages of T cells, including both
CD4+ and CD8+ subsets, increase with age and
that the CD4+/CD8+ ratio is unchanged across
age groups (30, 34). Our findings tend to differ with this
observation, as we found decreases in CD4+ T-cell
percentages and the CD4+/CD8+ ratio. Other
workers have also shown an elevated CD4+/CD8+
ratio in cord blood (7, 25) or in the first 5 years of life (5, 33). This is further supported by the results of studies of Japanese children by Yanase et al. (33) and Yachie et al. (32), who found a decreased
CD4+/CD8+ ratio as a result of an increased
percentage of CD8+ T-cell subsets and a decreased
percentage of CD4+ T-cell subsets over time. It is
reasonable to believe that this discrepancy between immunophenotype
patterns seen in Caucasian, Japanese, and Saudi Arabian populations may
be a reflection of significant differences in the relative
representation of CD8+ cells in T-cell subsets
(20), which could be due to the influence of the racial and
ethnic background. We have demonstrated in another study that healthy
Saudi Arabian male blood donors have a significantly higher percentage
and number of CD8+ T cells and a lower
CD4+/CD8+ ratio than healthy Caucasian males
(23). Several studies have demonstrated the different
influences of racial and environmental factors on the human lymphocyte
immunophenotype (20, 22, 27-29).
B cells, which were found to decline with age in our study, were
reported to show no age-related changes by Osugi et al.
(17). The same workers reported that the NK cell percentage
increased significantly with age, whereas it remained unchanged in our
study. In two other studies, the NK cell percentage was reported to
decline with time (9, 10). These different findings may also
be attributed to the influence of racial and environmental factors.
HLA-DR is an activation marker on T cells. There is a significant
increase in the percentage of HLA-DR+ T cells, whereas
there is a little change in their number, over time in this study. Most
of the earlier reports support our findings (9, 12, 34).
In conclusion, the data presented in this report confirm and extend the
findings on age-related changes in human blood lymphocyte subsets
reported earlier. Absolute and percentage values for most lymphocyte
subsets in healthy adults differ significantly from those for children.
Most importantly, among children, lymphocyte subsets vary significantly
with age. In addition, racial and environmental factors may have some
influence on the lymphocyte immunophenotype of children.
Therefore, when evaluating the immune status of children, consideration
of age-related changes along with racial and environmental factors
should be taken into account. The findings of this study are important
for interpreting changes in various diseases, including infections
which occur in children of different age groups.
| |
ACKNOWLEDGMENTS |
We thank Ibrahim Awad El Kareem for technical assistance, Amir
Marzouk for help with statistical analysis, and Vivian Darusin for
invaluable assistance in the preparation of this manuscript.
| |
FOOTNOTES |
*
Corresponding author. Present address: Allergy & Clinical Immunology Division, Johns Hopkins Asthma and Allergy Center,
Johns Hopkins University School of Medicine, 5501 Hopkins Bayview
Circle, Baltimore, MD 21224. Phone: (410) 550-2139. Fax: (410)
550-2130. E-mail: shahab{at}welchlink.welch.jhu.edu.
| |
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Clinical and Diagnostic Laboratory Immunology, September 1998, p. 632-635, Vol. 5, No. 5
1071-412X/98/$04.00+0
Copyright © 1998, American Society for Microbiology. All rights reserved.
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Abstract
Introduction
