Ralf Nass, MD; Suzan S. Pezzoli, BA; Mary Clancy Oliveri, MS; James T. Patrie, MS; Frank E. Harrell, PhD; Jody L. Clasey, PhD; Steven B. Heymsfield, MD; Mark A. Bach, MD; Mary Lee Vance, MD; Michael O. Thorner, MB, BS, DSc
Grant Support: By National Institutes of Health grants DK-32632 (Dr. Thorner) and RR-00847 (GCRC). Dr. Nass was supported in part by a grant from Deutsche Forschungsgemeinschaft (Na 317/1-1, Na 317/1-2). Merck Research Laboratories provided MK-677 and placebo. Additional support for assays was provided by grants NIH P30-DK 56336 (University of Alabama at Birmingham, Birmingham, Alabama) and NIH PO1-DK42618 (Columbia University, New York, New York).
Acknowledgment: The authors thank Mark L. Hartman, MD, and Arthur Weltman, PhD, for their contributions; Stephanie Studenski, MD, MPH, and Bette Ann Harris, DPT, MS, for review of the strength and function data; and Sue Brown, MD, for review of the bone data. They also thank Michael Johnson, PhD, and Paula Veldhuis for analysis of pulsatile GH secretion; Isao Eto, PhD; Alexandra Vyazovkina; Barbara Gower, PhD; Timothy R. Nagy, PhD; Jack Wang; and Jean Bergeron, MD, for laboratory work; and Shigehiro Oishi, PhD, for quality-of-life analyses. Finally, the authors thank the GCRC staff for care of our volunteers and the nurses; the Core Laboratory and Metabolic Kitchen personnel; and the staff of the Exercise Physiology Laboratory for performing body composition, strength, and function testing.
Potential Financial Conflicts of Interest:Employment: S.B. Heymsfield (Merck), M.A. Bach (Merck). Consultancies: M.O. Thorner (Merck). Honoraria: M.O. Thorner (Ipsen, Tercica, University of California Los Angeles, Duke University, New York Academy of Arts and Sciences). Stock ownership or options (other than mutual funds): M.A. Bach (Merck). Grants received: M.O. Thorner (National Institutes of Health, Bristol-Myers Squibb). Patents received: M.A. Bach (Merck). Patents pending: M.O. Thorner (methods for treating sarcopenia with a growth hormone secretagogue).
Reproducible Research Statement:Study protocol and statistical code: Available from Dr. Thorner (email@example.com). Data set: Not available.
Requests for Single Reprints: Michael O. Thorner, MB, BS, DSc, Department of Medicine, Box 801411, University of Virginia Health System, 450 Ray C. Hunt Drive, Aurbach Building, Room 2323, Charlottesville, VA 22908; e-mail, firstname.lastname@example.org.
Current Author Addresses: Drs. Nass and Thorner, Ms. Pezzoli, and Ms. Oliveri: Department of Medicine, Box 801411, University of Virginia Health System, 450 Ray C. Hunt Drive, Aurbach Building, Room 2323, Charlottesville, VA 22908.
Mr. Patrie: Department of Public Health Sciences, University of Virginia Health System, Box 800717, Charlottesville, VA 22908.
Dr. Harrell: Department of Biostatistics, Vanderbilt University School of Medicine, S2323 MCN, 1161 21st Avenue South, Nashville, TN, 37235.
Dr. Clasey: Department of Kinesiology and Health Promotion, University of Kentucky, 216 Seaton Center, Lexington, KY 40506.
Drs. Heymsfield and Bach: Merck Research Laboratories, 126 East Lincoln Avenue, Rahway, NJ 07065.
Dr. Vance: Department of Medicine, University of Virginia Health System, Box 800601, Charlottesville, VA 22908.
Author Contributions: Conception and design: R. Nass, S.S. Pezzoli, F.E. Harrell, M.A. Bach, M.L. Vance, J.L. Clasey, M.O. Thorner.
Analysis and interpretation of the data: R. Nass, S.S. Pezzoli, J.T. Patrie, F.E. Harrell, J.L. Clasey, S.B. Heymsfield, M.O. Thorner.
Drafting of the article: R. Nass, S.S. Pezzoli, J.T. Patrie, M.L. Vance, M.O. Thorner.
Critical revision of the article for important intellectual content: R. Nass, S.S. Pezzoli, J.T. Patrie, S.B. Heymsfield, M.A. Bach, M.L. Vance, M.O. Thorner.
Final approval of the article: R. Nass, S.S. Pezzoli, M. C. Oliveri, J.T. Patrie, F.E. Harrell, J.L. Clasey, S.B. Heymsfield, M.A. Bach, M.L. Vance, M.O. Thorner.
Provision of study materials or patients: R. Nass, M.C. Oliveri, M.O. Thorner.
Statistical expertise: J.T. Patrie, F.E. Harrell.
Obtaining of funding: M.A. Bach, M.O. Thorner.
Administrative, technical, or logistic support: R. Nass, S.S. Pezzoli, M.C. Oliveri, M.L. Vance, M.O. Thorner.
Collection and assembly of data: R. Nass, S.S. Pezzoli, M.C. Oliveri, M.L. Vance, M.O. Thorner.
ClinicalTrials.gov registration number: NCT00474279.
Nass R, Pezzoli SS, Oliveri MC, Patrie JT, Harrell FE, Clasey JL, et al. Effects of an Oral Ghrelin Mimetic on Body Composition and Clinical Outcomes in Healthy Older Adults: A Randomized Trial. Ann Intern Med. 2008;149:601-611. doi: 10.7326/0003-4819-149-9-200811040-00003
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Published: Ann Intern Med. 2008;149(9):601-611.
The age-related decline of growth hormone secretion may play a role in sarcopenia and frailty.
In this randomized trial, 65 healthy older adults were assigned to receive placebo or MK-677, an oral ghrelin mimetic that increased pulsatile growth hormone secretion to young-adult levels. Over 1 year, lean fat-free mass increased 1.1 kg with MK-677 and decreased 0.5 kg with placebo. MK-677 did not affect strength and function, but insulin sensitivity declined and mean serum glucose levels increased 0.28 mmol/L (5 mg/dL).
This short-term trial was underpowered to detect functional changes and adverse events.
An oral ghrelin mimetic increases pulsatile growth hormone secretion and alters body composition in healthy older adults.
Aging is an inevitable process across all species. In humans, muscle mass declines after reaching its peak in the third decade of life. Muscle mass is important for physical fitness and metabolic regulation; sarcopenia is a major risk factor for frailty, loss of independence, and physical disability in elderly persons (1) and is associated with shortened survival in critically ill patients (2). As lifespans increase, more adults are becoming frail and dependent on others, which creates challenges for them, their families, and society.
The decrease in fat-free mass correlates with the aging-associated decrease in growth hormone secretion (3, 4). Aging adults show decreases in fat-free mass and growth hormone secretion similar to those seen in growth hormonedeficient young adults (5). By the eighth decade, men and women lose approximately 7 and 3.8 kg of muscle mass, respectively (3), and gain intra-abdominal fat (6, 7).
Previous trials in which growth hormone was administered to elderly persons were small, poorly controlled, or too short (8); in addition, growth hormone replacement does not restore pulsatile growth hormone secretion. MK-677, the first orally active ghrelin mimetic (a growth hormone secretagogue and growth hormone secretagoguereceptor agonist), increases pulsatile growth hormone secretion in older adults to levels observed in young adults (9, 10). Our primary objectives were to determine whether 25 mg of oral MK-677 daily would increase growth hormone and insulin-like growth factor I (IGF-I) levels in healthy older adults, prevent the decline in fat-free mass, and decrease abdominal visceral fat, with acceptable tolerability.
The General Clinical Research Center (GCRC) and the University of Virginia institutional review boards approved this study. All participants gave written informed consent. We performed a 2-year, randomized, double-blind, modified crossover trial in which healthy older men, women receiving hormone replacement therapy, and women not receiving hormone replacement therapy received oral MK-677, 25 mg, or placebo (in a 2:1 ratio) daily. After 1 year, participants receiving MK-677 were randomly assigned to continue receiving MK-677 (group 1) or change to placebo (group 2); participants receiving placebo were given MK-677 during year 2 (group 3). Appendix Figure 1 shows the study design.
We recruited healthy volunteers older than 60 years of age from the general population by advertisement and screened them by medical history, physical examination, and laboratory testing to rule out underlying disease. Exclusion criteria were body mass index greater than 35 kg/m2, strenuous exercise for more than 60 minutes per day, smoking, diabetes, history of cancer (other than some types of skin cancer), untreated hypertension or thyroid disease, or medications known to affect growth hormone secretion. We asked participants to maintain their typical diet and exercise throughout the study and to report any illnesses, medical procedures, or adverse effects. All participants were white, with the exception of 1 Hispanic and 1 African-American man.
At baseline and every 6 months for 2 years, we admitted participants to the GCRC for measurement of body composition, body water, lipids, and bone mineral density; frequent blood sampling; and completion of quality-of-life questionnaires. We also performed tests of strength and function. During GCRC admissions, we standardized meals for caloric and nutrient content. Blood samples for growth hormone were drawn through an indwelling venous cannula every 10 minutes for 24 hours; participants were allowed to sleep after 9 p.m.
MK-677 and placebo tablets were provided by Merck Research Laboratories (Rahway, New Jersey) in a blinded manner and stored by a research pharmacist and dispensed in a blinded manner according to a randomization table with stratification for sex and hormone replacement therapy. Ten-mg tablets were provided for blinded back-titration. Participants were instructed to take the placebo or MK-677 tablets once daily between 7:00 and 9:00 a.m. (or at 9:00 a.m. during admissions). All research staff and volunteers remained blinded throughout the study and during data verification. We monitored adherence by pill counts.
We measured serum growth hormone and IGF-I levels in duplicate in the GCRC Core Laboratory. We assessed 24-hour mean growth hormone and endogenous growth hormone secretory dynamics by using the cluster method (11) and an automated multiple-parameter deconvolution method (9, 12). The Appendix provides details of all assay methods.
We evaluated fat-free mass and total body fat by using a 4-compartment model (13) and dual x-ray absorptiometry (DXA) on a Hologic QDR-2000 (Hologic, Bedford, Massachusetts) in pencil-beam mode (14). Dual x-ray absorptiometry measurements included appendicular lean soft tissue of the arms and legs as an estimate of total appendicular skeletal muscle mass (TASM) (15); appendicular fat; and bone mineral density of the femoral neck, spine (L2L4), and total hip.
We divided the DXA TASM estimates by height in square meters (TASM [kg]/m2) (15). We used this index of relative limb muscle mass to compute a T-score for each individual, relating the TASM/m2 to that of sex-concordant young adults (16). We defined sarcopenia as values more than 2 SD below values in young, sex-specific reference populations (17, 18).
We used cross-sectional computed tomographic images to measure the areas of abdominal visceral and subcutaneous fat and midthigh skeletal muscle at predefined anatomical locations (19); we excluded data if the subsequent scan location differed or we had technical difficulties (4 placebo group recipients and 3 MK-677 recipients). One blinded observer analyzed the dual x-ray absorptiometry and computed tomographic scans.
We measured total body water by using the deuterium oxide dilution technique (20) and extracellular water by using bromide dilution (21). We assessed intracellular water as the difference between total body water and extracellular water. To determine the relative relationships among total, extracellular, and intracellular water, we expressed each component in terms of kilograms of fat-free mass at each point. We chose the scale of measure for the analysis a priori. We also report the raw data in typical units for comparison.
We determined concentric force during flexion and extension of the knee and shoulder every 6 months by using a Cybex II isokinetic dynamometer (CSM, Boston, Massachusetts). Participants performed 6 repetitions of maximal effort over 90 degrees at 60 degrees/s, and the mean of the last 5 repetitions was computed by using proprietary software (22). We calculated total work by multiplying the mean per repetition by 5.
Function tests performed every 6 months included walking 30 meters as quickly as possible (best of 2 trials), walking as far as possible in 6 minutes on an indoor track, descending and ascending 4 flights of stairs, and rising and sitting 5 times from an armless chair with an 18-inch seat height.
To compensate for differences in muscle mass between men and women, we analyzed all strength and function measurements in terms of kilograms of baseline appendicular skeletal muscle (lean) from DXA. We used arm lean and leg lean for shoulder and knee strength, respectively, and baseline TASM (sum of arms and legs) for the function tests. We chose the scale of measure used in this analysis a priori; the raw data are also reported.
Participants completed 4 questionnaires every 6 months to assess quality of life and general well-being: the 20-item Short Form Health Survey, the Beck Depression Inventory, the Pittsburgh Sleep Quality Index, and the Body Cathexis Scale. The Appendix provides additional details of quality of life, muscle strength, and function assessments.
We measured cholesterol, cortisol, and insulin sensitivity (estimated by the Quicki Index method  from fasting insulin and glucose) every 6 months.
To determine whether the effects of MK-677 treatment were sustained for 2 years or reversed when changed to placebo, we analyzed several end points in a subgroup of participants who completed 24 months in each of the 3 treatment groups (Figure 1).
FBG= fasting blood glucose; HRT= hormone replacement therapy; MI= myocardial infarction.
Each year, volunteers were seen monthly for the first 3 months and every 3 months thereafter for a physical examination, documentation of medications and vital signs, and questioning about side effects and overall well-being. We performed a complete blood count and chemistry panel and monitored levels of hemoglobin A1c (HbA1c) and fasting blood glucose in all participants and prostate-specific antigen and testosterone in men. Women received annual Papanicolaou smears and mammography.
The 2 primary end points were fat-free mass and abdominal visceral fat. The study was powered for the pivotal first 12 months; the Appendix describes the power analysis in detail. We did not know whether men, women receiving hormone replacement therapy, and women not receiving hormone replacement therapy would respond differently. Consequently, we conducted the random assignments a priori so that equal numbers of these 3 populations would be assigned to MK-677 and placebo. We therefore focused the power analyses on the pivotal 12-month change comparison between the 2 treatment groups as a whole and not on specific subgroup comparisons, such as sex or hormone replacement therapy.
We conducted all statistical analyses under the guidelines of the intention-to-treat principle and did not impute missing data points. We performed the analyses on the baseline and the 6- and 12-month primary and secondary outcomes and decided the data analysis plan a priori. We used repeated-measures analysis of covariance to analyze the primary outcome data for the 6- and 12-month changes in fat-free mass, abdominal visceral fat, and IGF-I and growth hormone levels. For each analysis of covariance, we considered treatment (MK-677 or placebo), time (6 or 12 months), and treatment-by-time interaction to be potential sources of variability. We used the participants' baseline measurements as the analysis of covariance covariate. We analyzed the fat-free mass and abdominal visceral fat data in the same scale on which we measured them and report them as a difference between arithmetic means. We transformed the growth hormone and IGF-I data to the natural logarithmic scale before conducting the statistical analyses so that the variance and normality assumptions of the linear model were not violated and report the results as a ratio of geometric means (fold change).
We constructed linear contrasts to estimate the mean intraparticipant change in response at 6 and at 12 months and to estimate the baseline-adjusted difference in change in response at 6 and 12 months between the MK-677 and placebo groups. For the pivotal 12-month comparison (MK-677 versus placebo), we rejected the null hypothesis of equality of means if the P value of the F statistic was less than 0.05. For the 6-month between-group comparison, we rejected the null hypothesis if the P value of the F statistic was less than 0.05 after implementing the Bonferroni post hoc test correction. For the 12-month comparison, we constructed the 95% CI on the basis of the t test distribution quantile values at the 2.5 and 97.5 percentiles, whereas the 6-month comparison was based on the 1.25 and 98.75 percentiles of the distribution. With the exception of the quality-of-life data, we analyzed all secondary outcome data by using repeated-measure analysis of covariance and report them exactly as the primary outcome data. For the quality-of-life data, we performed a factor analysis (24) of the different scales of the questionnaires to create an overall well-being factor; the Appendix describes this in detail.
We designated the effects of year-2 treatment as exploratory. We performed a separate post hoc analysis of end points based on responses in year 1 to determine whether the effects were maintained or reversed in participants who had complete data at baseline, 12, and 24 months. We analyzed only the change from baseline to 24 months, in the same way as the year 1 data, and implemented a post hoc correction for the 3 treatment groups. We used SAS, version 9.1 (SAS Institute, Cary, North Carolina), to conduct the statistical analyses.
Additional methods, baseline data, and all results are presented in the supplementary appendix materials. Data are presented as means (95% CIs). All statistical comparisons at 6 and 12 months are between MK-677 and placebo.
This investigator-initiated GCRC study was funded by the National Institutes of Health and conducted and analyzed at the University of Virginia. All decisions regarding the design, conduct, analysis, and submission of the manuscript were made independently by the authors.
Figure 1 shows the flow of study participants, and the Table shows baseline demographic characteristics.
Treatment occurred between September 1998 and November 2003. Because the study drug expired in November 2003, 6 participants received treatment for only 18 months (2 placebo recipients and 4 MK-677 recipients) and 1 for only 12 months (placebo recipient). Seventy-one volunteers were randomly assigned; 65 participants (dropout rate, 8.5%) completed year 1: 23 men, 25 women receiving hormone replacement therapy, and 17 women not receiving hormone replacement therapy. The treatment groups were well matched at baseline, with no significant differences between groups. Fifty-nine participants completed 18 months and 53 completed 24 months of treatment (Figure 1).
In 4 participants, we blindly back-titrated the dose of study drug to 10 mg/d because of increased fasting glucose level after crossover from placebo to MK-677 in year 2 (an 81-year-old man who completed 2 years); increased fasting glucose level in 1 woman receiving MK-677 (withdrawn after 3 months); and increased joint pain in 2 women receiving MK-677 (withdrew after 12 months).
Figure 2 shows the effects of treatment in the pivotal year 1. After 12 months of MK-677 treatment, 24-hour mean growth hormone levels increased 1.8-fold (CI, 1.56- to 2.0-fold) from baseline (P < 0.001). This was accounted for by enhanced pulsatile growth hormone secretion (Appendix Table 1), as shown in a representative participant (Figure 2, C). Serum IGF-I levels also increased by 1.5-fold (CI, 1.4- to 1.6-fold; P <0.001). In 22 of 43 participants, IGF-I levels were sustained in the normal range for young adults; Appendix Figure 2 shows individual IGF-I results.
Growth hormone and IGF-I data were not normally distributed and were analyzed on the natural logarithmic scale. Line graphs show geometric means and 95% CIs. Results of growth hormone deconvolution analysis are included in Appendix Table 1. A. Mean 24-hour GH levels. The dashed line indicates 24-hour mean GH level for young men and women combined (~1.3 g/L). *P < 0.001 for MK-677 versus placebo. B. Serum IGF-I levels. The lower dotted line indicates the lower limit of the IGF-I normal range for older adults (59 to 225 g/L), and the upper dashed line indicates the lower limit in adults age 21 to 25 years (116 to 358 g/L). C. Representative 24-hour GH profile in a 70-year-old man with a body mass index of 23.2 kg/m2 who received MK-677 for 1 year. His 24-hour mean GH levels were 0.37, 1.0, and 0.86 g/L at baseline, 6 months, and 12 months, respectively. The pulsatile pattern of GH secretion at baseline is maintained and enhanced at 6 and 12 months, primarily because of increased secretion per peak rather than peak frequency.
Fat-free mass measured by DXA decreased in the placebo group and increased in the MK-677 group (change, 0.5 kg [CI, 1.10 to 0.2 kg] vs. 1.1 kg [CI, 0.7 to 1.5 kg], respectively; P < 0.001) (Figure 3, A). This increase was observed with both DXA and the 4-compartment model (R2= 0.98). Total appendicular skeletal muscle mass (limb lean) decreased in the placebo group and increased in the MK-677 group (change, 0.3 kg [CI, 0.6 to 0.1 kg] vs. 0.5 kg [CI, 0.3 to 0.8 kg], respectively; P <0.001).
Graphs show arithmetic differences (95% CI). Asterisks indicates a significant difference (MK-677 vs. placebo) at 12 months. 4-C= 4-compartment model; CT= computed tomography; DXA= dual energy x-ray absorptiometry; ECW= extracellular water; FFM= fat-free mass; ICW= intracellular water; SC= subcutaneous; TASM= total appendicular skeletal mass; TBW= total body water. A. Changes in FFM (by 4-C model and by DXA) and TASM (by DXA). B. Changes in TBW, EBW, and ICW. The increase in TBW and ICW with MK-677 are consistent with the anabolic effects of the drug. C. Changes in abdominal visceral and abdominal SC fat cross-sectional areas by computed tomography. D. Changes in body weight and total fat by 4-C model and DXA.
Thigh muscle area by computed tomography changed by 0.5 cm2 (CI, 3.2 to 2.2 cm2) in the placebo group and 1.5 cm2 (CI, 0.5 to 3.5 cm2; P= 0.20) in the MK-677 group (Appendix Table 2).
When each body water compartment was expressed per fat-free mass at each point, treatment groups did not differ significantly (Appendix Table 3).
Total body water increased by 0.1 kg (CI, 0.7 to 0.9 kg) in the placebo group and 1.7 kg (1.2 to 2.3 kg) in the MK-677 group (P= 0.001). Both groups had similar increases in extracellular water (placebo, 1.0 kg [CI, 0.02 to 2.1 kg]; MK-677, 1.0 kg [CI, 0.2 to 1.7 kg]). Intracellular water decreased in the placebo group but increased in the MK-677 group (change, 1.0 kg [CI, 2.1 to 0.2 kg] vs. 0.8 kg [CI, 0.1 to 1.6 kg], respectively; P= 0.021) (Figure 3, B). The loss of intracellular water or cell mass in the placebo group is reflected in a loss of total fat-free mass (Figure 3, A), specifically TASM. Conversely, the increase in cell mass in the MK-677 group is reflected in the significant increase in total fat-free mass and TASM (Figure 3, A).
Abdominal visceral fat increased 4.2 cm2 (CI, 6.2 to 14.5 cm2) in the placebo group and 8.4 cm2 (CI, 1.6 to 15.3 cm2) in the MK-677 group (P= 0.68) (Figure 3, C). Abdominal subcutaneous fat increased 1.3 cm2 (CI, 12.5 to 15.0 cm2) in the placebo group and 18.0 cm2 (CI, 8.7 to 27.2 cm2) in the MK-677 group (P= 0.054).
Body weight increased 0.8 kg (CI, 0.3 to 1.8 kg) in the placebo group and 2.7 kg (CI, 2.0 to 3.5 kg) in the MK-677 group (P= 0.003) (Figure 3, D). Total body fat by DXA increased 1.1 kg (CI, 0.2 to 1.9 kg) in the placebo group and 1.8 kg (CI, 1.2 to 2.5 kg) in the MK-677 group (P= 0.130).
Figure 4 compares the mean changes in limb lean and limb fat as they relate to the mean changes in fat-free mass and total fat mass in both groups. Placebo recipients lost limb lean, whereas about 50% of the increase in fat-free mass in MK-677 recipients was in the limbs. The average increase in limb fat in the MK-677 group was greater than that in the placebo group (1.1 kg vs. 0.24 kg; P= 0.001).
Limb= appendicular lean soft tissue and appendicular fat; nonlimb= total minus limb.
Appendix Figure 3 shows individual T-scores for TASM/m2 at baseline and 12 months. After 1 year, the T-score improved in 27 of 43 (63%) MK-677 recipients (mean, 0.29 [CI, 0.16 to 0.42]), whereas 18 of 22 (82%) placebo recipients experienced no change or a decrease in T-score (mean, 0.13 [0.32 to 0.06]; P <0.001).
After 12 months, femoral neck bone mineral density increased in the placebo group and decreased in the MK-677 group (change, 0.012 g/cm2 [CI, 0.002 to 0.022 g/cm2 vs. 0.005 g/cm2 [CI, 0.012 to 0.002 g/cm2], respectively). The difference between the MK-677 and placebo groups was small but significant (0.018 g/cm2; P= 0.004). Spine and total hip bone mineral density did not significantly differ. We observed the same pattern after excluding 5 participants receiving alendronate (3 MK-677 recipients and 2 placebo recipients).
Appendix Tables 2 to 4 show the detailed effects on other body composition end points and bone mineral density.
Shoulder flexion total work decreased in the placebo group but not in the MK-677 group. When we corrected for baseline arm appendicular skeletal muscle mass, shoulder flexion total work decreased more in the placebo group than the MK-677 group (change, 5.7 Nm/kg [CI, 10.1 to 1.4 Nm/kg] vs. 1.0 Nm/kg [CI, 4.1 to 2.1 Nm/kg]; P= 0.073). Total work in knee extension or flexion or in shoulder extension did not significantly differ between groups (Appendix Table 5).
No measure of function (Appendix Table 6) or quality of life (Appendix) significantly changed when the 2 groups were compared.
At 12 months, low-density lipoprotein cholesterol levels changed by 0.12 mmol/L (CI, 0.07 to 0.3 mmol/L; 4.6 mg/dL [CI, 2.7 to 11.6 mg/dL]) in the placebo group but 0.14 mmol/L (CI, 0.27 to 0.01 mmol/L; 5.4 mg/dL [CI, 10.4 to 0.4 mg/dL]; P= 0.026) in the MK-677 group. Total and high-density lipoprotein cholesterol levels did not differ between groups (Appendix Table 7).
Twenty-four-hour mean cortisol concentrations decreased in the placebo group (change, 18 nmol/L [CI, 55 to 19 nmol/L]; 0.1 g/dL [CI, 1.4 to 1.2 g/dL]) but increased in the MK-677 group (change, 47 nmol/L (CI, 28 to 71 nmol/L; 2.0 g/dL [CI, 1.0 to 2.9 g/dL]; P= 0.020) (Appendix Table 7).
Total testosterone levels in men did not change (Appendix Table 7). Prostate-specific antigen levels remained in the normal range or decreased with MK-677 treatment, except for a transient increase in 1 man. Results of mammography, Papanicolaou smears, and routine laboratory tests did not change over 2 years.
Appendix Figure 4 shows individual glucose and HbA1c responses. Mean fasting blood glucose levels did not change in the placebo group (0.0 mmol/L [CI, 0.3 to 0.2 mmol/L]; 1.0 mg/dL [CI, 5.0 to 3.0 mg/dL]) and increased 0.3 mmol/L (CI, 0.1 to 0.4 mmol/L; 5.0 mg/dL [CI, 2.0 to 7.0 mg/dL]; P= 0.015) in the MK-677 group. In 2 placebo recipients and 16 MK-677 recipients, fasting glucose increased from less than 5.6 mmol/L to 5.6 to 6.1 mmol/L [101 to 110 mg/dL]. In 3 MK-677 recipients with baseline fasting glucose concentrations less than 5.6 mmol/L [100 mg/dL] and 3 with concentrations greater than 5.6 mmol/L, glucose levels increased to 6.1 to 6.7 mmol/L (110 to 120 mg/dL) in 4 participants and to 6.9 mmol/L (125 and 126 mg/dL) in 2 participants. Mean HbA1c level decreased in the placebo group and increased in the MK-677 group (change, 0.1% [CI, 0.2% to 1.0%] vs. 0.2% [CI, 0.1% to 0.3%], respectively; P= 0.002); at 12 months, 8 participants had an HbA1c level greater than 6% (6.1% in 4, 6.3% in 3, and 6.4% in 1). Insulin sensitivity, as estimated by the Quicki Index, was also reduced after 12 months of treatment (P <0.001) (Appendix Table 8). One 81-year-old man had an increase in fasting blood glucose and HbA1c levels after crossing over from placebo to MK-677; after dose reduction and institution of a low-carbohydrate diet, the values returned to normal.
Eight of 22 (36%) placebo recipients reported an increase in appetite, compared with 29 of 43 (67%) MK-677 recipients (P= 0.033); appetite returned to normal in 3 months in 50% of MK-677 recipients and more gradually in others. Participants in both groups reported mild, transient edema (6 of 22 [27%] placebo recipients vs. 19 of 43 [44%] MK-677 recipients; P= 0.30); transient muscle pain (2 of 22 [9%] placebo recipients vs. 14 of 43 [33%] MK-677 recipients; P= 0.076); and joint pain (17 of 22 [77%] placebo recipients vs. 25 of 43 [58%] MK-677 recipients; P= 0.20).
In year 1, adenocarcinoma of the tongue was diagnosed at 12 months in an 82-year-old woman receiving MK-677, and a 68-year-old woman had a myocardial infarction 7 days after starting MK-677. Renal cell carcinoma was diagnosed at 6 months in 1 man receiving placebo. All were withdrawn from the study. At the end of year 2, colon cancer was diagnosed in an 83-year-old woman who received MK-677 in year 1 and placebo in year 2.
Two-year exploratory analyses of changes from baseline to 24 months in a subgroup of 53 participants (Appendix Table 9) confirmed that the significant changes observed in the pivotal first year were sustained for growth hormone and IGF-I levels (Appendix Figure 5), fat-free mass (by DXA only), and T-score for TASM/m2 (Appendix Figure 6). Appendix Figure 7 shows changes in body weight, total fat mass, fasting blood glucose levels, and abdominal visceral fat. In the group treated for 2 years with MK-677, fasting blood glucose level was not significantly increased (P= 0.093 vs. baseline).
We observed similar changes in participants who received MK-677 in year 2 after placebo in year 1 (group 3), whereas the changes were reversed in those who received MK-677 in year 1 and placebo in year 2 (group 2). One month after crossover and at 3 and 6 months after study completion, IGF-I concentrations returned to pretreatment levels.
Healthy elderly persons who received the ghrelin mimetic MK-677 experienced a sustained increase in the amplitude of pulsatile growth hormone secretion and IGF-I levels to those seen in young adults. The likely mechanism was activation of the ghrelin receptor by MK-677, with feedback by IGF-I preventing excess growth hormone production. MK-677 increased fat-free mass by 1.6 kg relative to placebo. To provide perspective, an adult's average lifetime loss of fat-free mass is about 5.5 kg (3). The concomitant increase in intracellular water, which reflects body cell mass (25), was probably the mechanism for the increase in fat-free mass.
Ghrelin stimulates growth hormone secretion, but it also has effects that are not attributable to increased growth hormone levels. A ghrelin mimetic transiently increases appetite, a novel effect that might counteract physiologic anorexia, a cause of weight loss in elderly persons (26, 27). Unlike growth hormone, which is lipolytic, ghrelin increases fat stores. We found that body weight increased more in MK-677 recipients than in placebo recipients. Although total fat mass increased in both groups, limb fat and limb lean mass increased more in participants receiving MK-677 than in those receiving placebo. Surprisingly, thigh muscle cross-sectional area did not increase, although our study was not powered to detect small but potentially important differences because the single-slice computed tomography method that we used was insufficiently precise. Growth hormone reduces abdominal visceral fat in growth hormonedeficient adults (28) and abdominally obese, postmenopausal women (29) but not in normal elderly participants (30). Although MK-677 increased growth hormone levels, it did not affect abdominal visceral fat, possibly because its combined orexigenic and adipogenic effects counteracted the lipolytic effects of enhanced growth hormone. Finally, although MK-677 did not reduce abdominal visceral fat, it did reduce low-density lipoprotein cholesterol levels at 12 months, an effect not seen with growth hormone in normal elderly participants (8).
Strength, function, and quality of life did not improve after administration of MK-677 in our small, healthy cohorta result we should possibly have expected. Although strength improved in elderly patients with hypopituitarism after daily injections of growth hormone for 2 to 3 years (31), growth hormone alone does not increase strength in healthy elderly persons (8, 32, 33). Strength improved only in healthy older men receiving growth hormone plus testosterone for 26 weeks (33). Finally, the relationship between strength and physical performance is nonlinear (34); we speculate that increased physical capacity might substantially improve performance in frail adults but not healthy adults.
Sarcopenia is a hallmark of frailty (35, 36) and is associated with increased mortality in elderly persons (3740). In our healthy sample, MK-677 counteracted 3 important factors that contribute to sarcopenia: reduced secretion of growth hormone, loss of fat-free mass, and inadequate food intake. We did not study patients with sarcopenia, and their response to a ghrelin mimetic is not known.
Of note, our participants tolerated daily administration of MK-677 for the 2-year study period. The most frequent side effects were mild, transient, lower-extremity edema; transient muscle pain; and increased appetite, which subsided in a few months. These effects of physiologically stimulated growth hormone secretion contrast with those of growth hormone administered by injection: edema, arthralgia, carpal tunnel syndrome, gynecomastia, and new-onset impaired fasting glucose and diabetes mellitus in some persons (8).
Both growth hormone and MK-677 increase insulin resistance and blood glucose in elderly persons (22, 33, 41, 42). We found statistically significant but small increases in fasting blood glucose and HbA1c levels at 12 months. Considering the results of short-term studies with MK-677 (9, 43), which found no statistically significant increase in serum cortisol, the small increase in serum cortisol that we found is unlikely to underlie the increase in fasting glucose level. In patients treated with growth hormone, bone mineral density initially decreases (44); at least 18 months of treatment is needed to demonstrate an increase in bone mineral density (45). Femoral neck bone mineral density decreased at 12 months in MK-677 recipients, which is consistent with the increased bone remodeling that occurs with growth hormone (44). Fracture risk is the best measure of the effects of MK-677 on bone; however, this outcome would require studies of large samples over many years.
Our study has limitations. Its duration was relatively short, and the sample was small. Combining the results for men and women may have missed important sex effects. As a small, randomized study in healthy older adults, ours was a proof-of-concept study. It showed, apparently for the first time, that a drug can maintain the IGF-I levels and physiologic pattern of growth hormone secretion seen in young adults for at least 1 year and partially reverse age-related body composition changes.
Frailty is one of the scourges of elderly persons, and as researchers are beginning to learn about its causes, they are asking whether growth hormone deficiency is one of them. A systematic review (8) concluded that the risks of exogenous growth hormone outweigh the benefits and that it is not the long-sought solution to frailty. The promise of MK-677 is that it seems to restore endogenous growth hormone levels in a physiologic secretory pattern, unlike the single high-amplitude pulse observed after exogenous growth hormone administration. We believe that our study sets the stage for an adequately powered clinical trial of sufficient duration in a population vulnerable to frailty.
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Feinberg School of Medicine of Northwestern University
November 12, 2008
Strategies for remaining as healthy adults
The study by Nass et. al. (1) elegantly reinforces the prevalent health strategy first proposed by an immigrant, Juan Ponce De Leon, in 1513 (2). Simply find the magic fountain, or the right pill, and perpetual youth and perhaps even immortality will be yours, without breaking a sweat, and oh, don't worry about the cost. A contrasting approach would cite the impressive data confirming the benefits of lifestyle changes, especially exercise, in preventing and reversing frailty, (3) which as a bonus reduces obesity, prevents falls and may even improve mental status. All this without decreasing insulin sensitivity or other potential long term side effects such as diabetes.
Perhaps any future studies testing ghrelin mimetic should include a "control group" using an aerobic and weight resistance exercise program combined with a diet intervention. One might reasonably predict that this latter group would outperform the pharmacologically enhanced cohort by a wide margin. They would also feel better and have lower costs while only expending sweat equity.
1. Nass R, Pezolli SS, Olivero JT; et. al. Effects of oral ghrelin mimetic on body composition and clinical outcomes in healthy older adults. A randomized trial. Ann Intern Med. 2008;149:601-611
2. Olschki, L. Ponce De Leon's fountain of youth: History of a geographical Myth. The Hispanic Historical Review. Duke University Press, 1941. Durham NC. Vol XXVI #3 pp 361-385 3. Hall W. Centenarians: Metaphor becomes reality. Arch Intern Med. 2008;168:262-263
Dept. of Rheumatology, Kaiser Franz Josef Hospital, Vienna, Austria
To proof a concept of a drug without side effects
To the editors: I read with interest the study done by Nass et al (1), however, I want to address some critical issues with particular reference to adverse events: First, there is growing evidence, that IGF-1 is a cytokine involved in promotion and induction of oncogenesis in different types of tumors, as Ewing's sarcoma(rev. in 2) , Renal cell carcinoma (3), adenocarcinoma of the GI tract (e.g. colorectal carcinoma (4) and cholangiocellular carcinoma). I wonder why the authors do not report the results of screening methods (FOBT, abdominal ultrasound, colonoscopy) or staging of reported AEÂ´s. Second, MRI-imaging and biopsy of skeletal muscle in relation to the observed effects would have been of interest in context with a clinical trial trying to prove a concept. And finally, I think, that the study didn't focus on adverse events or economic issues as told in the objective. But, I wish I would have read a detailed discussion of the observed AEÂ´s. Non-pharmacologic treatment strategies for decreased muscle strength and increased (intra-) abdominal fat in the elderly have to be mentioned when talking about sarcopenia and increased blood glucose levels.
1. Nass R, et. al. Effects of oral ghrelin mimetic on body composition and clinical outcomes in healthy older adults. A randomized trial. Ann Intern Med. 2008;149:601-611
2. Cironi L, et al. (2008) PLoS ONE 3(7): e2634. doi:10.1371/journal.pone.0002634
3. Jungwirth A, et al. Proc Natl Acad Sci U S A. 1997; 94(11):5810-3
4. Simmons JG et al. Am J Physiol Gastrointest Liver Physiol. 2007; 293(5): G995"“1003.
Universidad Nacional AutÃ³noma de MÃ©xico
November 13, 2008
Aging process is a disease
I read with interest the article by Nass and colleagues (1) in which the authors presented some clinical evidences of rejuvenation on 65 healthy older adults (men and women) ranging from 60 to 81 years of age, after daily administration of oral ghrelin (secretagogue product) during 1 year. Oral administration of MK-677 increased pulsatile growth hormone (GH)secretion and increased serum Insulin-like growth factor I(IGF-I, also known as somatomedin C) levels (2). In part, I agree with these authors,because through the blood flow the GH secretagogues (constituted by a combination of aminoacids, some peptides, vitamines and minerals) may reach to the producing hypothalamic nuclei of growth hormone-releasing hormone (GHRH) (3) and thus, increase the GH secretion from the adenohypophysis. However, these results may fail on older persons due to atherosclerotic plaques located at the mouths of the collateral branches originated from the supraclinoid carotids and circle of Willis (3,4 ). In contrast, a revascularization of the arcuate nucleus and surrounding nuclei by means of omental tissue can provoke rejuvenation (3), because through the omentum, the hypothalamus receives an increase in blood flow, oxygen, neurotransmitters, neurotrophic factors, cytokines and omental stem cells (3,5). For these reasons, I have postulated that aging is not a normal biological process but a disease.
1. Nass R,Pezzoli SS,Oliveri Co, et al.Effects of an oral ghrelin mimetic on body composition and clinical outcomes in healthy older adults. Ann Inter Med 2008;149(9):601-611.
2. Chapman IM,Bach MA,Cauter E,et al.Stimulation of the growth(GH)-insulin-like growth factor I axis by daily oral administration of a GH secretagogues(MK-677)in healthy subjects. J Clin Endocrinol Metab 1996;81:4249-4257.
3. Rafael H. Rejuvenation after omental transplantation on the optic chiasma and carotid bifurcation. Case Rep Clin Pract Rev 2006;7:48-51.www.amjcaserep.com
4. Rafael H. Hypothalamic ischemia and premature aging.Med Sci Monit 2007;13(7):LE9-10. www.medscimonit.com 5-Garcia-Gomez I,Goldsmith HS,Angulo J,et al.Angiogenic capacity of human omental stem cells. Neurol Res 2005;27(8):807-811.
Michael O. Thorner
University of Virginia Health System
December 15, 2008
Effects of an Oral Ghrelin Mimetic on Body Composition and Clinical Outcomes in Healthy Older Adults
We appreciate the thoughtful comments offered in response to our paper and offer some clarifications.
We believe that aging is not a disease, but a complex multi-system decline that occurs over decades. It is likely that MK-677 acts at multiple sites, including the hypothalamus, the pituitary and the periphery. We have no evidence that atherosclerosis impairs its action.
We did not perform other cancer screening in these healthy older adults. Subjects were carefully monitored with Pap smears and mammograms, as well as PSA levels in men. Adverse effects were reported in the results section. A study of this size cannot assess cancer risk, however, as of July 20, 2007 more than 600 adult patients had been exposed to MK-677 for 6-12 months. The combined incidence rate for malignancies in any MK-677 treatment group was similar to the incidence rate in the placebo groups in these studies (personal communication, Dimitris A. Papanicolaou). The cancer risk of growth hormone and IGF-I administration is controversial and has been extensively reviewed (1).
As outlined by Dr. Webster, the benefits of exercise are well established and always should be recommended. However, physiologic studies show that the effects of resistance training on intramuscular metabolic changes achieved in the elderly, as well as muscle growth response, are significantly lower when compared to a younger study population (2,3). Additional data suggest that in men over 80 years of age, the capacity to gain strength with resistance training is decreased because of the limited myocellular adaptive response.(4).
Furthermore, some elderly adults are not able to exercise because of significant muscle loss and frailty. Interventions that prevent or delay a decline in muscle mass would be desirable, given the expected demographic shift in the aging population. Our observations support a role for ghrelin mimetics to enhance growth hormone secretion; this resulted in both arrest of muscle mass loss, as well as an increase in muscle mass. The increase in appetite also may be important. Recent data from the Health ABC study demonstrate a significant association between change in lean mass in the elderly and dietary protein intake (5).
Long-term studies comparing the effects of exercise to a ghrelin mimetic alone or in combination with exercise are certainly needed in elderly subjects who are physically able to exercise. We emphasized that ours was a "˜proof-of-concept' study and now the definitive studies need to be designed and performed.
1. Consensus. Critical evaluation of the safety of recombinant human growth hormone administration: statement from the Growth Hormone Research Society. J. Clin. Endocrinol. Metab. 2001; 86:1868-1870. [PMID: 11344173]
2. Kosek DJ, Kim JS, Petrella JK, Cross JM, Bamman MM. Efficacy of 3 days/wk resistance training on myofiber hypertrophy and myogenic mechanisms in young vs. older adults. J Appl Physiol. 2006;101:531-544. [PMID: 16614355].
3. Welle S, Thornton C, Statt M. Myofibrillar protein synthesis in young and old human subjects after three months of resistance training. Am J Physiol. 1995;268:E422-E427. [PMID: 7900788].
4. Slivka D, Raue U, Hollon C, Minchev K, Trappe S. Single muscle fiber adaptations to resistance training in old (>80 yr) men: evidence for limited skeletal muscle plasticity. Am J Physiol 2008;295:R273-280. [PMID: 18448613].
5. Houston DK, Nicklas BJ, Ding J, Harris TB, Tylavsky FA, Newman AB et al. Protein intake is associated with lean mass change in older, community-dwelling adults: the Health, Aging, and Body Composition (Health ABC) Study. Am J Clin Nutr. 2008;87:150-155. [PMID: 17515911]
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