|
1990 Dr. Daniel Rudman Study
New England Journal of
Medicine, Volume
323 July 5, 1990 Number 1
EFFECTS OF HUMAN GROWTH HORMONE IN MEN OVER 60 YEARS OLD
Daniel Rudman, M.D., Axel G. Feller, M.D., Hoskote S. Nagraj,
M.D., Gregory A. Gergans, M.D., Pardee Y. Lalitha, M.D., Allen F. Goldberg,
D.D.S., Robert A. Schlenker, Ph.D., Lester Cohn, M.D., Inge
W. Rudman, B.S., and Dale E. Mattson, Ph.D.
Abstract Background.
The declining activity of the growth hormone-insulin-like growth factor 1
(IGF-1) axis with advancing age may contribute to the decrease in lean body
mass and the increase in mass of adipose tissue that occur with aging.
Methods. To
test this hypothesis, we studied IGF-1 plasma with 21 healthy men from 61 to
81 years old who had plasma IGF-1 concentrations of less than 350 U per
liter during a six-month base-line period and a six-month treatment period
that followed. During the treatment period, 12 men (group 1) received
approximately 0.03 mg of biosynthetic human growth hormone per kilogram of
body weight subcutaneously three times a week, and 9 men (group 2) received
no treatment. Plasma IGF-1 levels were measured monthly. At the end of each
period, we measured lean body mass, the mass of adipose tissue, skin
thickness (epidermis plus dermis), and bone density at nine skeletal sites.
Results. In
group 1, the mean plasma IGF-1 level rose into the youthful range of 500 to
1500 U per liter during treatment, whereas in group 2 it remained below 350
U per liter. The administration of human growth hormone for six months in
group 1 was accompanied by an 8.8 percent increase in lean body mass, a 14.4
percent decrease in adipose-tissue mass, and a 1.6 percent increase in
average lumbar vertebral bone density (P<0.05 in each instance). Skin
thickness increased .1 percent (P = 0.0). There was no significant change in
the bone density of the radius or proximal femur. In group 2 there was no
significant change in lean body mass, the mass of adipose tissue, skin
thickness, or bone density during treatment.
Conclusions.
Diminished secretion of growth hormone is responsible in part for the
decrease of lean body mass, the expansion of adipose-tissue mass, and the
thinning of the skin that occurs in old age. (New England Journal of
Medicine, 1990; 323:1-6).
In middle and late adulthood,
all people experience a series of progressive alterations in body
composition. The lean body mass shrinks and the mass of adipose tissue
expands. The contraction in lean body mass reflects atrophic processes in
skeletal muscle, liver, kidney, spleen, skin, and bone.
These structural changes have
been considered unavoidable results of aging. It has recently been proposed,
however, that reduced availability of growth hormone in late adulthood may
contribute to such changes. This proposal is based on two lines of evidence.
First, after about the age of 30, the secretion of growth hormone by the
pituitary gland tends to decline. Since growth hormone is secreted in
pulses, mostly during the early hours of sleep, it is difficult to measure
the 24-hour secretion of the substance directly. Growth hormone secretion
can be measured indirectly, however measure the 24-hour secretion of the
substance measure the 24-hour secretion of the substance directly. Growth
hormone secretion can be measured indirectly, however, by measuring the
plasma concentration of insulin-like growth factor I (IGF-I, also known as
somatomedin C), which is produced and released by the liver and perhaps
other tissues in response to growth hormone. There is little diurnal
variation in the plasma IGF-I concentration, and measurements of it are
therefore a convenient indicator of growth hormone secretion. Plasma IGF-I
concentrations decline with advancing age in healthy adults. Less than 5
percent of the healthy men 20 to 40 years old have plasma IGF-I values of
less than 350 U per liter, but the values are below this figure in 30
percent of the healthy men over 60. Likewise, the nocturnal pulses of growth
hormone secretion becomes smaller or disappear with advanced age. If the
plasma concentration of IGF-I falls below 350 U per liter in older adults,
no spontaneous circulating pulses of growth hormone can be detected by
currently available radioimmunoassay methods. The concomitant decline in
plasma concentrations of both hormones supports the view that the decrease
in IGF-I results from diminished growth hormone secretion. Second,
diminished secretion of growth hormone is accompanied not only by a fall in
the plasma IGF-I concentration, but also by atrophy of the lean body mass
and expansion of the mass of adipose tissue. These alterations in body
composition caused by growth hormone deficiency can be reversed by
replacement doses of the hormone, as experiments in rodents, children, and
adults 20 to 50 years old have shown. These findings suggest that the
atrophy of the lean body mass and its component organs and the enlargement
of the mass of adipose tissue that are characteristic of the elderly result
at least in part from diminished secretion of growth hormone. If so, the
age-related changes in body composition should be correctable in part by the
administration of human growth hormone, now readily available as a
biosynthetic product.
In this study we administered
biosynthetic human growth hormone for six months to 12 healthy men from 61
to 81 years old whose plasma IGF-I concentrations were below 350 U per
liter, and we measured the effects on plasma IGF-I concentration, lean boy
mass, adipose-tissue mass, skin (dermal plus epidermal) thickness, regional
bone density, and mandibular-height ratio (the height of the alveolar ridge
divided by the total height of the mandible). In addition, the men were
monitored for possible adverse effects of the hormone by means of interviews
physical examinations, and standard laboratory tests. Nine men matched for
age and with similar plasma IGF-I concentrations served as controls.
Methods
Subjects
Healthy men who were 61 or
older and living in the community were recruited through newspaper
advertisements followed by an interview. Entry criteria (available from the
authors on request) included body weight of 90 to 120 percent of the
standard for age, the ability to administer growth hormone to oneself
subcutaneously, and the absence of indications of major disease. Ninety-five
men who answered the advertisement met criteria that could be ascertained by
interview. Their plasma IGF-I concentrations were then determined twice at
an interval of four weeks Consistent with the results of a previous study,
the plasma IGF-I values in these men ranged from 100 to 2400 U per liter,
with an average of 500 U per liter. Thirty- three of the men had plasma IGF-I
values of less than 350 U per liter on both occasions. These 33 men were
then further evaluated by a medical-history taking, physical examination,
differential blood count, urinalysis, blood-chemistry tests, chest
radiography, and electrocardiography. Twenty-six subjects (1 black and 25
white) met all the entry criteria and were enrolled in the 12-month protocol
summarized in Table 1.
Study Periods
The men were seen at regular
intervals and tested as shown in Table 1 during the first week of the first,
third, and sixth months of the base-line period. Five men dropped out of the
study during these six months (four for personal reasons and one because
carcinoma of the prostate was detected).
Table 1. Schedule of Tests During the Base-Line and Treatment
Periods
SUNDAY, JUNE 16, 1990 7:08:56 AM SUNDAY, JUNE 16, 1990 7:08:56 AM
SUNDAY, JUNE 16, 1990 7:08:56 AM
| Test |
Base
Line Period |
Treatment
Period |
| |
Mo |
Mo |
Mo |
Mo |
Mo |
Mo |
Mo |
Mo |
Mo |
| |
1 |
3 |
6 |
7 |
8 |
9 |
10 |
11 |
12 |
| Physical
Examination |
x |
x |
x |
x |
x |
x |
x |
x |
x |
| Hematology* |
x |
x |
x |
x |
x |
x |
x |
x |
x |
| Urinalysis* |
x |
x |
x |
x |
x |
x |
x |
x |
x |
| Blood
Chemistry* |
x |
x |
x |
x |
x |
x |
x |
x |
x |
| Chest
radiography |
x |
|
x |
|
|
|
|
|
x |
| Electrocardiography |
x |
|
x |
|
|
|
|
|
x |
| Echocardiography |
x |
|
x |
|
|
|
|
|
x |
| Total
body potassium† |
|
|
x |
|
|
|
|
|
x |
| Skin
thickness‡ |
|
|
x |
|
|
|
|
|
x |
| Bone
density*Š |
|
|
x |
|
|
|
|
|
x |
| Mandibular-heightratio*þ` |
|
|
x |
|
|
|
|
|
x |
| Plasma
IFG1¶ |
x |
x |
x |
x |
x |
x |
x |
x |
x |
| Biosynthecic
growth hormone** |
|
|
|
x |
x |
x |
x |
x |
x |
†
Total body potassium levels (lean body mass and adipose tissue-mass) were
measured according to the method of Flynn et al. 15
‡ Calculated at the sum of skin
thickness of the right and left dorsal hand and left volar forearm measured
with a Harpenden caliper according to the method of Lawrence and Shuster.16
*Š Measured according to the method of
Nagraj et al.17
*þ` Measured according to the method of
Goldberg et al.18
¶ Measured at Nichols Laboratory, Los
Angeles, according to the method of Furlanetto et al.19
** Administered to group 1 only.
At the beginning of the seventh
month, the 21 men who had completed the base-line period were randomly
assigned to group 1 (growth hormone group) or group 2 (control group) in a
ratio of 3 to 2. The randomization table was generated by a computer program
such that in each group of five men, three would be assigned to the growth
hormone group and two to the control group. All 21 men (12 in group 1 and 9
in group 2) completed the treatment period and continue the study group for
this report. Their clinical characteristics are summarized in Table 2.
During the first week of the seventh month, the men in group 1 were
instructed in the subcuntaneious administration of recombinant biosynthetic
human growth hormone (2.6 IU per milligram of hormone; Eli Lilly). The
initial dose was 0.03 mg per kilogram of body weight, injected three times a
week at 8a.m., the interval between injections being either one or two days.
A sample of venious blood for plasma IGF-I assay was obtained each month 24
hours after a growth hormone injection. If the IGF-I level was below 500 U
per liter, the dose of hormone w as increased by 25 percent; if the IGF-I
level was above 1500 U per liter, the dose was reduced by 25 percent. The
men in group 2 received no injections. The schedule of tests of both groups
during the treatment period is shown in Table 1.
At the start of the base-line
period, the project dietician instructed each man to follow a diet that
furnished 25 to 30 k.cal per kilogram. The distribution of kilocalories
among protein, carbohydrate, and fat was approximately 15 percent, 50
percent, and 35 percent, respectively. At each scheduled visit shown in
Table 1, the dietitian analyzed each man's diet on the basis of a 24-hours
dietary recall and instructed the subjects again about the standard diet.
The men were told not to alter their lifestyles (including their use of
tobacco or alcohol and their level or physical activity) during the 12-month
study period.
The study protocol was carried
out with the informed consent of each subject and with the approval of the
human-research committees of the Medical College of Wisconsin, the Chicago
Medical School, and the Veterans Affairs Medical Centers in North Chicago
and Milwaukee.
Table 2. Clinical
Characteristics of the Study Subjects.
| Characteristic |
Group1
(N=12) |
Group2
(N=9) |
| Median age
(range) |
67 (61-73) |
68 (65-81) |
| Percent of
ideal body weight- -median (range) |
103
(94-120) |
105
(99-117) |
| |
|
|
| Medical
conditions (no. of subjects) |
|
|
| Degenerative
joint disease |
5 |
2 |
| Benign
prostatic hypertrophy |
3 |
1 |
| Glaucoma |
1 |
1 |
| Cataract |
2 |
1 |
| Arterioscleotic
heart disease* |
3 |
1 |
| Gallstones |
0 |
1 |
| Kidney
stone |
1 |
1 |
| Hiatus
hernia |
0 |
1 |
| |
| Medications
(no. of subjects) |
|
|
| Nonsteroidal
antiinflamitory drug |
3 |
1 |
| Pilocarpine
eyedrops |
1 |
1 |
| Cimetidine |
0 |
1 |
*
Defined as history of myocardial infraction or electrocardiographic
abnormality ascribed to coronary artery disease.
Statistical
Analysis
The methods used to measure
each response variable and the locations where the tests were performed are
described in Table 1. The interassay coeficients of variation for the
response variables were as follows: plasma IGF-I, 7.2 percent; lean body
mass, 3.6 percent; adipose-tissue mass, 6.9 percent; skin thickness, 5.4
percent; and bone density, 2.3 percent (average of nine measured sites).
P values based on two-tailed
matched-pair t-tests were calculated for the comparisons between the 6-month
and 12-month values in group1 and group 2. In addition, for each response
variable the 6-month value was subtracted from the 12-month value to
represent the change in each subject. P values based on two-tailed,
unequalvariance, independent-sample t-tests were then calculated for the
comparison of the changes in response variables between groups 1 and 2.
Results
Clinical Observations
All the men remained healthy, and none had any changes in the results
of differential blood count, urinalysis, blood-chemistry profile, chest
radiography, electrocardiography, or echocardiography during the 12-month
protocol. Specifically, none had edema, fasting hyperglycemia (>6.6 mmol
of glucose per liter), an increase in blood pressure to more than 160/90 mm
Hg, ventricular hypertrophy, or a local reaction to human growth hormone,
nor did their serum cholesterol or triglyceride concentrations change
significantly. In group 1, however, both the men (" SE) systolic blood
pressure and fasting plasma glucose concentration were significantly higher
(P<0.05 by matched-pair t-test) at the end of the experimental period
than at the end of the base-line period (127.2"5.2 vs. 119.1"
3.6mm Hg and 5.8" 0.2 vs. 5.4" 0.2 mmol per liter, respectively).
Table 3. Effect of the Administration of Human Growth Hormone
on Plasma IGF-1 Concentrations in Healthy Older Men*
| |
Plasma
IGF-1 |
| |
Base
Line Period |
Treatment
Period |
| |
Mo 1 |
Mo. 3 |
Mo.6 |
Mo.7 |
Mo.8 |
| Group 1 |
240 +-86 |
230+-97 |
230+-66 |
830 +-339H |
680+-180H |
| |
Mo. 9 |
Mo.10 |
Mo.11 |
Mo.12 |
|
| |
720+-350H |
810+-305H |
810+-192H |
910+-312H |
|
| Group 2 |
Mo 1 |
Mo. 3 |
Mo. 6 |
Mo. 7 |
Mo.8 |
| |
240+-69 |
240+-126 |
240+-108 |
200+-126 |
220+-123 |
| |
Mo. 9 |
Mo.10 |
Mo.11 |
Mo.12 |
|
| |
240+-177 |
180+-126 |
240+-186 |
300+-201 |
|
*Values are means
+-SD HP<0.05 for the comparison between groups
Plasma IGF-I Concentration
In group 1, the mean plasma IGF-I
concentration ranged from 200 to 250 U per liter throughout the base-line
period (Table 3). Within one month after the administration of growth
hormone had been initiated, the mean IGF-I level rose to 830 U per liter
(P<0.05), and it remained near this value for the next five months. Eight
of the 12 men in group 1 required no adjustment in their initial dose of
growth hormone. Two required an upward adjustment of 25 percent, and two
required a downward adjustment of 25 percent. The mean plasma IGF-I
concentration in group 2 remained in the range of 180 to 300 U per liter
throughout the base-line and treatment periods.
Lean Body Mass, Adipose-Tissue
Mass, Skin Thickness, Bone Density and Mandibular-Height Ratio
Table 4 shows the mean values
for the other response variables at the end of the base-line period (6
months) and the end of the treatment period (12 months). There was no
significant change in weight in either group. In group 1, several response
variables had changed significantly after 12 months. Lean body mass and the
average density of the lumbar vertebrae increased by 8.8 percent
(P<0.0005) and 1.6 percent (P<0.04), respectively, and adipose-tissue
mass decreased by 14.4 percent (P<0.005). The sum of skin thicknesses at
four sites increased .1 percent (P = 0.07). The small average change in
lumbar vertebral bone density (only 0.02 g per square centimeter) was
statistically significant because of very little variability in individual
results. The bone density of the radius and proximal femur and the ratio of
the height of the alveolar ridge to total mandibular height did not change
significantly. In group 2 none of these variables changed significantly. The
change in the lean body mass was significantly greater in group 1 than in
group 2 (P<0.018), but the differences in changes in skin thickness and
adipose-tissue mass between groups did not reach statistical significance in
this small series (P = 0.10 and 0.13, respectively).
Table 4. Effect of the
Administration of Human Growth Hormone on Weight, Lean Body Mass,
Adipose-Tissue Mass, Skin Thickness, and Bone Density in Healthy Older Men
| Variable |
Group |
End of Base
Line Period |
End of Base
Line Period |
P ValueH |
Difference
in ChangesI |
| Weight (kg) |
1 2 |
77.2+-11.4
83.3+-11.1 |
78.2+-12.1
83.3+-9.7 |
0.26 0.97 |
+1.0 (-1.4
to 3.4) |
| Lean Body
Mass (kg) |
1 2 |
53.0+-7.4
54.2+-7.1 |
57.7+-9.1
55.2+-7.3 |
0.05 0.17 |
+3.7 (+0.7
to +6.6) |
| Adipose
Tissue Mass (kg) |
1 2 |
24.1+-5.0
29.0+-6.4 |
20.6+-5.6
28.0+-4.0 |
0.05 0.43 |
-2.4 (-5.7
to +0.8) |
| Sum of Skin
Thickness at four Sites (mm) |
1 2 |
9.9+-1.2
9.3+-0.9 |
10.6+-1.5
9.23+-0.80 |
0.07 0.69 |
+0.8 (-0.1
to +1.7) |
| Bone Density
(g/cm2) Mid-shaft radius |
1 2 |
0.74+-0.10
0.76+-0.10 |
0.74+-0.12
0.71+-0.07 |
0.85 0.09 |
+0.40 (-0.02
to +0.10) |
| Distal
radius |
1 2 |
0.37+-0.07
0.34+-0.04 |
0.36+-0.08
0.33+-0.05 |
0.12 0.26 |
-0.004
(-0.03 to +0.02) |
| Average
lumbar vertebrae 1-4 |
1 2 |
1.23+-0.12
1.29+-0.25 |
1.25+-0.13
1.29+-0.26 |
0.04 0.64 |
+0.006
(-0.04 to +0.05) |
| Ward's
Triangle |
1 2 |
0.70+-0.14
0.70+-0.17 |
0.69+-0.13
0.70+-0.17 |
0.15 0.69 |
-0.018
(-0.08 to +0.05) |
| Greater
trochanter |
1 2 |
0.85+-0.13
0.81+-0.15 |
0.85+-0.13
0.81+-0.13 |
0.72 0.55 |
+0.007
(-0.05 to +0.03) |
| Fremoral
neck |
1 2 |
0.92+-0.15
0.89+-0.14 |
0.91+-0.14
0.85+-0.14 |
0.53 0.14 |
-0.029
(-0.08 to +0.03) |
| Mandibular
height ratio |
1 2 |
0.45+-0.15
0.47+-0.12 |
0.46+-0.11
0.47+-0.12 |
0.87 0.98 |
-0.003
(-0.07 to +0.06) |
*
Plus-minus values are means +-SD
HP values are for
the change from base line, by matched pair 1-test
I The difference in
changes (12 month value minus 6 month value) is the average in group 1 minus
the average change in group 2. Values in parentheses are 95 percent
confidence intervals, calculated by independent-sample, unequal-variance
1-test.
Discussion
The 21 men studied were
representative of the approximately one third of all men 60 to 80 years old
who have plasma IGF-I concentrations of less than 350 U per liter (as
compared with a range of 500 to 1500 U per liter in healthy men 20 to 40
years old). Our findings cannot be generalized to the approximately two
thirds of all men over 60 who have plasma IGFK-I concentrations of more than
350 U per liter or to women of a similar age. Furthermore, our entry
criteria focused the study on an overly healthy subgroup of older men.
In the absence of obesity,
below-normal weight, or liver disease, a plasma IGF-I concentration of less
than 350 U per liter in older men generally signifies that they secrete very
little growth hormone. To verify this explanation for the low plasma IGF-I
concentration in these men, it would be necessary to measure serum growth
hormone levels at frequent intervals for 24 hours or to determine the
24-hour urinary excretion of growth hormone. We did not do this, but Ho et
al. found that the 24-hour integrated serum growth hormone level was
markedly lower in the men over 55 than in men 18 to 33 years old. An
alternative explanation for a low plasma IGF-I concentration is decreased
production of plasma IGF-I binding proteins. Most of the IGF-I plasma is
bound to these proteins, but their concentrations vary little in healthy
people who eat a normal diet.
In the 12 men in group 1,
initially low plasma IGF-I concentrations were raised to the normal range
for young adult men by the dose of growth hormone administered, with no
evidence of tachyphylaxis or hormone resistance. The dose, approximately
0.03 mg per kilogram three times a week, was based on published estimates of
the rate of growth hormone secretion in young men and was comparable to or
smaller than doses given previously to children with growth hormone
deficiency and young adults. The plasma IGF-I responses to this dose in
these older men were similar in magnitude to those in younger people. That
"replacement" rather than pharmacologic doses were being
administered was confirmed by the plasma IGF-I measurements, which remained
within the range for healthy young adults (500 to 1500 U per liter)
throughout the treatment period (Table 3). We conclude that in aging men
with low plasma IGF-I concentrations hepatic responsiveness to human growth
hormone is not impaired, and the decline in plasma IGF-1 concentrations in
such men results from growth hormone deficiency rather than growth hormone
resistance. The increase in plasma IGF-1 levels that occurs when growth
hormone is administered to children with growth hormone deficiency reflects
not only augmented hepatic production of IGF-1, but also increased
production of one of the binding proteins that transport IGF-1. The extent
to which the production of IGF-1 binding protein is increased by the
administration of growth hormone has not yet been studied in adults.
At the beginning of our study,
adverse reactions to human growth hormone were thought to be unlikely
because physiologic doses were being used. Furthermore, similar or larger
doses have not caused undesired reactions in children or young adults.
Nevertheless, it remained possible that this dose, when given for six months
to older subjects, might cause some manifestation of hypersomatotropism,
such as edema, hypertension, diabetes,k or cardiomegaly. Although none of
these conditions developed, there were small increases in the mean systolic
blood pressure and fasting plasma glucose concentration of the group of men
who received growth hormone.
The magnitude of the increases
in lean body mass and the decreases in adipose-tissue mass (8.8 and -14.2
percent above and below base line, respectively) in the aging men who
received human growth hormone for six months was similar to the magnitude of
these responses in children and young adults treated with similar or lower
doses for three to six months, a comparison that provides further evidence
that tissue responsiveness to growth hormone and IGFK-I is not altered in
older men. Until now, the evidence for such a conclusion came only from
short-term nitrogen-balance experiments.
Salomon et al. reported that
the administration of human growth hormone in a dose of 0.49 unit per
kilogram per week (0.19 mg per kilogram per week) for six months to adults
20 to 50 years old who had growth hormone deficiency lowered the serum
cholesterol concentration significantly. Serum cholesterol concentrations
did not change in our study, in which the does of growth hormone was about
half as large (0.9 mg per kilogram per week). The divergent results could
reflect differences in the subjects' ages, the degree of growth hormone
deficiency, the dose of hormone, or all three.
In rodents, the increase in
lean body mass in response to growth hormone is due to increases in the
volume of skeletal muscle, skin, liver, kidney, and spleen. In young human
subjects, an enlargement of muscle and kidney induced by growth hormone has
been documented, other organs have not yet been assessed. The reduction in
adipose-tissue mass when children with growth hormone deficiency are treated
with human growth hormone is associated with a redistribution of adipose
tissue from abdominal to peripheral areas. It is not known however, whether
the increase in lean body mass and the decrease in adipose-tissue mass are
qualitatively as well as quantitatively similar in old and young human
subjects.
Biosynthetic human growth
hormone had no detectable effect on the bone density of the radius or
proximal femur in the aging men but it increased the density of the lumbar
vertebrae by about 1.6 percent. Although the decrease in bone density with
advancing age in men may be due in part to diminished secretion of growth
hormone, longer periods of administration of human growth hormone will be
required before a final conclusion can be drawn regarding its efficacy in
reversing that decrease. A similar interpretation applies to the lack of
increase in the mandibular-height ratio.
The findings in this study are
consistent with the hypothesis that the decrease in lean body mass, the
increase in adipose-tissue mass, and the thinning of the skin that occur in
older men are caused in part by reduced activity of the growth hormone - IGF-I
axis, and can be restored in part by the administration of human growth
hormone. The effects of six months of human growth hormone on lean body mass
and adipose-tissue mass were equivalent in magnitude to the changes incurred
during 10 to 20 years of aging. Among the questions that remain to be
addressed are the following: What will be the benefits and what will be the
nature and frequency of any adverse effects when larger numbers of elderly
subjects and other doses of human growth hormones are studied? What organs
are responsible for the increase in lean body mass, and do their functional
capacities change as well? Only when such questions are answered can the
possible benefits of human growth hormone in the elderly be explored. Since
atrophy of muscle and skin contributes to the frailty of older people the
potential benefits of growth hormone merit continuing attention and
investigation.
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