Abstract
Introduction
The cystatin C (CysC) serum level is a marker of glomerular filtration rate and depends on age, gender, and pubertal stage. We hypothesize that CysC might overall reflect energy homeostasis and be regulated by components of the endocrine system and metabolites in pubertal adolescents.
Methods
Serum CysC levels and further possible effector parameters in 5355 fasting, morning venous blood samples from 2035 healthy participants of the LIFE Child cohort study (age 8 to 18 years) were analyzed. Recruitment started in 2011, with probands followed up once a year. Linear univariate and stepwise multivariate regression analyses were performed.
Results
Annual growth rate, serum levels of thyroid hormones, parathyroid hormone, insulin-like growth factor 1, hemoglobin A1c (HbA1c), uric acid, and alkaline phosphatase show relevant and significant associations with CysC serum concentrations (p <0.001). Furthermore, male probands’ CysC correlated with the body mass index and testosterone among other sexual hormones. Multivariate analyses revealed that uric acid and HbA1c are associated variables of CysC independent from gender (p <0.001). In males, alkaline phosphatase (p <0.001) is additionally significantly associated with CysC. Thyroid hormones show significant correlations only in multivariate analyses in females (p <0.001).
Conclusions
The described associations strongly suggest an impact of children’s metabolism on CysC serum levels. These alterations need to be considered in kidney diagnostics using CysC in adolescents. Additionally, further studies are needed on CysC in children.
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Introduction
Due to its function as an endogenous marker for the glomerular filtration rate (GFR) and thus kidney function, the cysteine protease inhibitor and low molecular weight protein cystatin C (CysC) is of high interest not only in pediatric nephrology [1]. As the product of a housekeeping gene, it is produced by all human nucleated cells at a stable rate [2]. Because it is freely filtered in the glomerulus, it correlates well with GFR determined by gold standard methods, such as the chromium-ethylenediaminetetraacetic acid complex (CrEDTA) or inulin in children and adults [3,4,5,6]. Measuring methods include the rapid and precise particle-enhanced turbidimetric and nephelometric immunoassays (PETIA and PENIA) [7, 8]. The studies of Yata et al. (n = 1128) and Groesbeck et al. (n = 719) first showed that CysC decreases in adolescents aged 15–16 years, being significantly higher in males compared to females at the same age [9, 10]. In our earlier studies, we were able to confirm these findings and proposed the usage of percentiles for the laboratory assessment of CysC in pediatric patients [11]. Whereas serum levels of female adolescents decrease starting at 11 years of age, those for male adolescents increase (ß = 0.028 mg/l/a) until the age of 15 years. From the age of 13 years, they differ significantly from one another [11]. Similar to creatinine, this difference amounts to 15% and is therefore of clinical relevance [10, 11]. Body height and pubertal stage, among others, are good predictors of the CysC serum level [11]. Recently, Miliku et al. suggested that GFR estimated by equations relying on CysC are negatively associated with body mass index (BMI) and body surface area (BSA), but not lean or fat mass percentage [12]. Whereas in adults, the effects of age, gender, height, and weight on CysC are well described [13], they are not satisfactorily assessed in children.
Underlying metabolic and hormonal influences may include blood glucose levels, insulin as well as glucocorticoids [14,15,16]. Additionally, thyroid dysfunction along with alteration of triiodothyronine (FT3), insulin-like growth factor 1 (IGF-1), and growth hormone (GH) levels are associated with serum CysC levels [17,18,19,20]. Further essential impacts on CysC were found in vitro in bone resorption excitatory as well as inhibitory activity [21, 22], uric acid in high school students [23], and serum albumin concentrations in both adults and children [13, 15]. We hypothesize age- and gender-specific correlations of CysC serum concentrations and these indicators of growth and metabolism in generally healthy adolescents [11]. Based on our earlier results, we assume that testosterone and anabolic hormones are significantly associated with CysC serum levels in boys and girls during puberty. Therefore, we aim to investigate potential associations of metabolic enzymes and hormones with serum CysC concentrations in adolescents.
Material and methods
Design and study population
Coherence with STROBE (Strengthening the Reporting of Observational Studies in Epidemiology) criteria is shown in annex [24]. The data were assessed within the LIFE Child study in the Leipzig Research Centre for Civilization Diseases (LIFE) [25, 26]. The population-based cohort study is recruiting primarily healthy infants, children, and adolescents in Leipzig (Germany) since 2011. We included measurements of all participants aged 8 to 18 years with valid CysC measurements. Up to 2019, the 2126 participants had one up to eight follow-up visits (once per year). We excluded those with kidney anomalies, nephrolithiasis, or febrile urinary tract infections in their medical history (n = 89). The respective diagnoses were obtained by computer-assisted personal interview and sonography diagnostic. Furthermore, we identified and excluded four remaining isolated extreme values of CysC (< 0.4 mg/l), most probably due to measurement errors. Therefore, our study includes 5355 observations of 2035 children in total.
The examinations were performed by trained medical staff following highly standardized procedures [25, 26]. To date, we were able to establish reference intervals for serum CysC levels [11], lipids [27], liver enzymes [28], iron-related blood parameters [29], and metabolites [30] in healthy children. Our study was conducted according to the Declaration of Helsinki and was approved by the Ethics Committee of the University of Leipzig (reg. no. 264-10-19042010), NCT trial number 02550236. All data are pseudomized to comply with the German data protection law and the General Data Protection Regulation of the European Union. More information about our cohort is described by Poulain et al. and Quante et al. [25, 26].
Laboratory assessment
CysC serum levels and all further laboratory parameters were analyzed in fasting morning venous blood drawn by venipuncture. The Institute for Laboratory Medicine, Clinical Chemistry and Molecular Diagnostic (ILM), University Hospital Leipzig, used an automated laboratory analyzer, Cobas8000 (Roche Diagnostics, Mannheim Germany), following the manufacturer’s protocol. The method used for CysC is the turbidimetric immunoassay (PETIA) Tina-quant® cystatin C (Roche Diagnostics). Primary measurement range is 0.4–8.0 mg/l. Detailed information can be found in Ziegelasch et al. [11]. Furthermore, Suppl. Table 1 summarizes the assessment of the other laboratory parameters along with the respective test, analyzer, and material examined.
Anthropometric assessment
The measurements of skin plication, weight, and height were taken by our trained staff following highly standardized procedures. The measurement devices, including a stadiometer (measurement accuracy of 0.1 cm) and a Seca 701 scale (measurement accuracy of 50 g), were regularly calibrated. The growth rate was calculated using the difference of height (last visit height subtracted from the current visit height) divided by time in days between two visits in our research center.
Statistics
Univariate and multivariate analyses were performed using the R software (version 4.0.0) [31]. For multivariate analyses, we used stepwise linear regression analyses (backward deletion) to determine the associations of the independent variables on CysC levels (R-package lme4 [32]). The heatmaps show pairwise correlations between CysC and potentially influencing variables in males and females through illustration of significance levels (p values). To account for multiple measurements per subject, the subjects were added as random effect on the intercept in all analyses. Furthermore, all analyses were corrected for age. It is noteworthy that cortisol and uric acid were only assessed in subcohorts with subjects selected by random sampling.
Results
In total, the data of 2035 participants with 5355 observations was analyzed. The descriptive data are shown in Table 1. Furthermore, the distributions of pubertal stages and BMI in the LIFE Child cohort are summarized in Table 2. Boys enter the pubertal stage II approximately half a year later than girls.
Results of univariate linear regression models
Table 3 and Fig. 1 show the results of the linear regression models for male and female subjects separately. Sex-independent results of the entire cohort are summarized in Suppl. Table 2. All analyses were corrected for age and repeated measurements per subject by adding the age and pseudonym as random effects.
In the entire study population, CysC is positively correlated with the growth rate as well as BMI (p <0.01). This effect can also be seen in the male subcohort. Additionally, in males, the puberty status (p <0.001), the iliac, triceps (p <0.05), and the subscapular skin folds in millimeters (p <0.001) are positively associated with CysC serum levels. Nevertheless, in the female subcohort, only growth rate, iliac skin plication, and pubertal status show significant associations (p <0.001).
Regarding the endocrine system, testosterone is positively and significantly associated with CysC in males (p <0.001), but negatively in females (p <0.01). Furthermore, in males, follicle-stimulating hormone (FSH) and luteinizing hormone (LH) correlate positively with serum concentrations of CysC (p <0.001), but with only a small effect size for LH. In females, FSH shows similar significant correlations with CysC, whereas LH and estradiol have only very small effect sizes. Of all thyroid hormones, FT3 and free thyroid hormone 4 (FT4) show inverse correlations with CysC (p <0.001). Besides, parathyroid hormone (PTH) is associated with serum CysC levels independently from gender, whereas no association with cortisol could be found. IGF1 and in males insulin are two further hormones that show significant correlations with CysC (p <0.001).
Metabolic enzymes and further parameters were investigated. Hemoglobin A1c (HbA1c) and in male probands the blood glucose level also correlate significantly with CysC serum concentrations (p <0.001). An association can also be seen with serum protein and gamma-glutamyl transferase in males as well as with albumin, urea, alanine-aminotransferase (ALAT, p <0.05), and aspartate-aminotransferase serum levels (ASAT, p <0.001) in female probands. Finally, uric acid and alkaline phosphatase are associated with serum CysC independent from gender (p <0.001).
Results of hierarchical multivariate regression models
In stepwise multivariate linear regression analysis (backward deletion), we determined the factors having the most significant statistical association and the highest effect size on CysC. All factors showing statistically significant effects on CysC in univariate linear regression models including anthropometric data were considered in the analyses. The results are shown in Table 4.
The final model for females includes the free thyroid hormones FT3 and FT4 (p <0.001) that are both inversely associated with CysC serum concentrations with ß = 0.0300 and ß = −0.0117, respectively. In addition, HbA1c (ß = −0.1026) and uric acid (ß = 0.5 × 10−3) show significant correlations (p <0.001).
In male participants, the last four remaining effector variables after stepwise deletion were the alkaline phosphatase (ß = 0.0165, p <0.001), HbA1c (ß = −0.1107, p <0.001), uric acid (ß = 0.0005, p <0.001), and testosterone (ß = 0.0021, p = 0.051).
Discussion
CysC levels were shown to be associated with height, age, and puberty [11], with puberty status being a strong predictor of CysC serum concentrations, especially in 11- to 14-year-old adolescents. This is coherent with previous studies [9, 10, 33]. Likewise, we found a positive correlation of pubertal status with CysC in boys and a negative correlation in girls. The growth rate is one strong predictor of serum CysC levels in all participants in univariate analyses. However, in the multivariate regression model, it does not exceed the effect of the factors described in Table 4. In contrast to girls, boys’ serum CysC concentrations are associated with the BMI. The effect of BMI has earlier been investigated by Alosco et al. before and 12 months after bariatric surgery, showing that BMI as well as CysC significantly decreased [34]. Another large study with more than 8000 adults showed that age, gender, weight, and height were associated with CysC levels [13]. Marmarinos et al. described an interaction of CysC and BMI. However, Miliku et al. found no correlation with the lean or fat mass percentage in 6-year-old children, but did not investigate children or adolescents during puberty [12, 33]. Overall, we assume an effect of body composition and development on CysC due to altering metabolism. This effect is most obvious in pubertal boys and may be explained by a higher growth rate compared to adolescent girls with an anabolic status.
Underlying hormonal mechanisms are already discussed in earlier studies: GH and FT3 enhance the production of CysC in adipocytes [18]. In vivo, FT3 enhances CysC levels in patients with hyperthyroidism [19]. When examining post-transsphenoidal surgery patients, CysC declined similarly to GH and IGF1 [20]. A positive correlation of FT3 is confirmed in our study, whereas FT4 is negatively associated with CysC. These two parameters are showing significant, but inverse associations with CysC serum concentrations in multivariate analyses in girls. The deiodinase may explain this inverse effect, although, to our knowledge, no studies investigating this potential association exist to date. Only in patients with thyroid dysfunction, CysC levels were already described to moderately but significantly rise along with thyroxin blood levels [17]. IGF-1 is another factor with relevant effect in both males and females, which, however, does not exceed the effect of the factors in the described multivariate analyses. One similarity of all these potential effector variables is their physiological function in the body’s metabolism and body growth.
After stepwise deletion in the multivariate analyses, testosterone was among the four remaining factors with the strongest correlations to serum CysC with a final ß of 0.505 (p = 0.051). To our knowledge, no studies examining this correlation to CysC in children exist so far. Veldhuis et al. only found lower estradiol and increased testosterone associated with higher IGF-I in healthy aging adults, suggesting IGF-1 as a potential mediator variable [35]. Nevertheless, Phillip et al. did not find any effects of testosterone on CysC when investigating hypophysectomized castrated rats [36]. Therefore, an association of testosterone and CysC may depend on the pituitary gland activity, maybe through activation of the GH axis.
In our study, the anabolic hormone insulin showed a significant correlation to CysC only in males. Therefore, insulin may be another potential mediator or effector in the interdependence of CysC and pubertal stage in boys. Testosterone induces an anabolic metabolism that may result in an increasing insulin serum level. Meanwhile, no relevant effect of the metabolic hormone cortisol on CysC could be found. So far, only studies in children treated with glucocorticoids for malignancy or kidney disease were proven to have elevated levels of serum CysC [14,15,16]. An interaction of glucocorticoid levels and CysC is not described in healthy children yet.
Finally, we examined the association of indicators of cell and body metabolism with CysC. Lerner and Grubb described a positive correlation of CysC with bone resorption as well as its potential function of antagonizing the effect of PTH and PTH-related peptide on bone metabolism [22]. The accumulation of CysC in milk basic protein in vitro was positively correlated to osteoblastic proliferation as well as bone resorption inhibitory activity in a study by Yasueda et al. [21], confirming the findings of Lerner and Grubb. In our study, PTH was associated with CysC with ß = 0.017 (p <0.001) independent from gender. On the contrary, alkaline phosphatase as an indicator of bone metabolism remained one potential effector variable of CysC in multivariate analyses in boys, not in girls. Nevertheless, the effect does not differ between boys and girls in univariate analyses (ßboys = 0.022 and ßgirls = 0.025, both p <0.001). We assume that alkaline phosphatase may increase especially in pubertal boys with an elevated growth rate compared to girls. Other potential indicators of cell metabolism, i.e., cellular processes of degradation and new formation, include uric acid, whose direct correlation with CysC was shown to be higher in boys than girls [23]. Likewise, serum albumin concentrations are known to be associated with lower concentrations of CysC [13, 15]. We found uric acid to be a strong predictor of serum CysC levels in both males and females, even in multivariate analyses (ß = 0.005, p <0.001), whereas serum albumin concentrations showed no relevant impact on CysC. However, uric acid was only assessed in subcohorts with subjects selected by random sampling (n = 1237). The high correlation with CysC in multivariate analyses may be explained by the physiological role of uric acid in cell metabolism as mentioned above. Additionally, uric acid is renally excreted and therefore depends on kidney function with CysC as an important indicator.
The metabolic function of the liver may also alter CysC serum concentrations: associations with the matrix metalloproteinase 2 and hepatic diseases both positively correlated with CysC [37]. Furthermore, a direct correlation with liver fibrosis stages and the severity of liver diseases was found [38,39,40]. However, associations of liver enzymes and CysC in primarily healthy subjects were not described yet. We found only low associations with ASAT and ALAT, as well as urea in girls, with gamma-glutamyl transferase in boys. They may indicate increased metabolic activity in pubertal adolescents, although this potential interdependence would not explain the differences between boys and girls found in this study.
Limitations of this study include the methodology: CysC concentrations were assessed by turbidimetric assays, whereas a previous meta-analysis favors nephelometric assays [41]. The different methodology may explain discrepancies of our results with those of other studies. Furthermore, correlation does not necessarily mean a causal relationship between cystatin C and the considered variable. Causality may for example be determined by Mendelian randomization studies. Besides, the homogeneity of our primarily Caucasian cohort of Leipzig limits the generalizability of the results.
Overall, we assume that body growth in boys due to pubertal development affects the synthesis of the housekeeping protein CysC. Its positive correlation with testosterone and alkaline phosphatase as predictors of body growth underline this thesis. The underlying mechanisms may include the hormonal stimulation of the body’s cell metabolism. This may also explain the high accuracy of eGFR equations such as the Andersen formula including the body cell mass [42, 43].
Conclusions
The results show that differences in CysC during puberty are associated with testosterone and other indicators of cell metabolism and growth. Due to the broad age range from 8 to 18 years, a large number of observations (n = 5335) of healthy participants, and a standardized assessment, the results are of high accuracy. They emphasize the necessity of using percentiles of CysC serum levels in adolescents in kidney diagnostics. Additionally, further studies are needed on CysC in children.
Data availability
All data generated or analyzed during this study are included in this published article and its supplementary information files.
Code availability
The R scripts are available in this article’s supplementary information files.
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Acknowledgements
The authors gratefully acknowledge all the participants and their families for their cooperation and participation in the LIFE Child study. Additionally, we appreciate the dedicated contributions of the LIFE Child study team.
Funding
Open Access funding enabled and organized by Projekt DEAL. The Leipzig Research Centre for Civilization Diseases was funded by the European Union, the European Regional Development Fund as well as the Free State of Saxony within the framework of the excellence initiative of the Saxonian Ministry of Science and Arts (SMWK), Free State of Saxony, Germany (NCT trial number: 02550236 (NIH)).
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Niels Ziegelasch: conceptualization, methodology, formal analysis, original draft, visualization, Mandy Vogel: formal analysis, data curation, validation, software, review and editing, visualization, Antje Körner: conceptualization, methodology, review and editing, Eva Koch: conceptualization, investigation, resources, Anne Jurkutat: conceptualization, investigation, resources, Uta Ceglarek: conceptualization, methodology, validation, formal analysis, review and editing, Katalin Dittrich: conceptualization, methodology, review and editing, supervision, Wieland Kiess: conceptualization, methodology, review and editing, supervision, project administration, funding acquisition.
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Ziegelasch, N., Vogel, M., Körner, A. et al. Cystatin C relates to metabolism in healthy, pubertal adolescents. Pediatr Nephrol 37, 423–432 (2022). https://doi.org/10.1007/s00467-021-05209-2
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DOI: https://doi.org/10.1007/s00467-021-05209-2