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Fenretinide Breast Cancer Prevention Trial

Drug and Retinol Plasma Levels in Relation to Age and Disease Outcome¹

Istituto Nazionale Tumori, 20133 Milan, [F.F., T.C., E.C., V.A., M.G.V., G.D.P., M.G.D.M.]; S. Maugeri Foundation, Pavia [A.C.]; and Istituto Europeo di Oncologia, 20133 Milan [U.V.], Italy

	Abstract

Top Abstract Introduction Patients and Methods Results Discussion References

 
Objectives: To assess, in women participating in a breast cancer prevention trialon fenretinide (4-HPR), the relationship of drug and retinol levels with the risk of second breast malignancy, taking into account age and menopausal status.

Methods: In a multicenter prevention trial, women with early breast cancer were randomly assigned to receive no treatment or 200 mg of 4-HPR/day for 5 years. Blood was collected at baseline and on a yearly basis during intervention from women recruited at the Istituto Tumori (Milan, Italy; 818 and 756 in the 4-HPR and control arm, respectively, who accounted for 53% of the participants in the trial). The plasma concentrations of 4-HPR, its main metabolite N-(4-methoxyphenyl) retinamide, and retinol were assayed by high-performance liquid chromatography. Three age ranges (45, 46–55, and 56 years), menopausal status at baseline, and disease outcome at a median follow-up of 97 months were taken into account in the analysis.

Results: Baseline retinol levels were significantly lower (P 0.05) in subjects 45 years than in older subjects, and among subjects in the age range 46–55 years, they were significantly higher (P 0.001) in those in postmenopause than in those in premenopause. Baseline retinol levels were not related to the risk of a second breast malignancy. 4-HPR and N-(4-methoxyphenyl)retinamide levels were not affected by menopausal status. They slightly, but significantly (P 0.05), increased with age (46 years versus 45 years) but only in disease-free subjects. Among subjects < 45 years, they were slightly, but significantly (P 0.05), higher in those subjects in which breast cancer recurred. 4-HPR treatment caused a retinol level reduction, which was strongly (r 0.71; P 0.001) related to pretreatment retinol levels.

Conclusions: Retinol plasma levels increased with age and after menopause and were not related to breast cancer recurrence. 4-HPR levels were lower in subjects < 45 years than in older subjects. The inverse relationship between drug plasma levels and 4-HPR preventive effects observed in young women suggests a role for 4-HPR plasma sequestration in 4-HPR biological activity.

	Introduction

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In March 1987, a multicenter randomized trial was started to assess the efficacy of the synthetic retinoid 4-HPR³ as a breast cancer preventive agent (1) . The objective of the trial was to evaluate the efficacy of a 5-year intervention with 4-HPR versus no treatment in reducing the incidence of contralateral breast cancer or ipsilateral breast cancer in women operated on for early breast cancer. A different effect of 4-HPR was found depending on menopausal status, with a possible beneficial effect in premenopausal women and a reverse trend in postmenopausal women.

Similarly, studies on subgroups of women participating in the prevention trial had shown that 4-HPR affected circulating insulin-like growth factor-1 differently depending on age, with a greater reduction in women 50 years (mostly in premenopause) than in older women (2 , 3) . All together, these findings suggest an interaction between 4-HPR effects and menopausal status or age.

Information on 4-HPR pharmacokinetics and pharmacodynamics was obtained during a Phase I study, which was run to identify the dose to be administered in the breast cancer prevention study (4 , 5) . We demonstrated that 4-HPR, administered at 200 mg/day, resulted in average 4-HPR and 4-MPR plasma levels of 1 µM, which remained constant over the 5-year treatment period (4) and caused a 70% decrease in plasma retinol levels (4 , 5) . In these studies, because of the few patients investigated, it was not possible to assess the potential influence of age or menopausal status on 4-HPR pharmacokinetics. Now with the availability of measurements of drug and retinol levels in plasma samples collected at baseline and during intervention from 1574 women (818 and 756 in the 4-HPR and control arm, respectively) participating in the Phase III prevention trial, it seemed appropriate to evaluate the association between drug plasma levels and disease outcome, taking into account the age and menopausal status of the patients. Moreover, because few and contradictory results (6, 7, 8, 9, 10) have been reported on the potential association between vitamin A (or retinol) and breast cancer, we assessed whether prerandomization or on-study retinol levels were predictive of breast cancer risk and recurrence.

	Patients and Methods

Top Abstract Introduction Patients and Methods Results Discussion References

 
Sample Population and Treatment.
The sample population of the study consisted of 1574 women (818 in the 4-HPR arm and 756 in the control arm, see Table 1 ) participating in a multicenter 4-HPR breast tumor prevention trial (1) . The women were those followed at the Istituto Nazionale Tumori, Milan, Italy, and they accounted for 53% of the participants in the trial. The median follow-up duration for clinical response is the same as the prevention trial, i.e., 97 months. Blood samples from 83 women (blood donors: age range 28–67 years), with no evidence of a breast tumor, were also collected and analyzed for comparison of retinol levels.

Sample Collection and Analytical Procedure.
Subjects allocated to the 4-HPR arm had plasma samples collected before randomization (at baseline) and periodically during follow-up visits (at least every 12 months) during the 5 years of study. Subjects allocated to the control arm had plasma collected at baseline and after 5 years. For each sample, the interval from randomization (in months) was reported. For samples of the 4-HPR arm, the interval (in h) from the last dose and the number of capsules taken (one or two) were also reported.

Blood was collected in heparinized tubes and wrapped in aluminum foil; all procedures were performed in the dark. After centrifugation, separated plasma was kept frozen at -20°C until analysis, never >3 weeks. Aliquots of 0.2 ml of plasma were added to 0.4 ml of CH₃CN containing butylated hydroxytoluene (125 µg/ml; Sigma, St. Louis, MO) as antioxidant, and the concentrations of 4-HPR, 4-MPR, and retinol were detected by high-performance liquid chromatography as described previously (4) . The reference standards 4-HPR (molecular weight, M_r 391,000) and 4-MPR (molecular weight, M_r 405,000) were supplied by the R.W. Johnson Pharmaceutical Research Institute; retinol, used as reference standard, was obtained from Sigma.

Statistical Analysis.
Menopausal status (before or after menopause), defined as the absence of menstruation for 1 year (1) , and age at baseline were considered. Preliminary studies were performed on the relationship of retinol, 4-HPR, and 4-MPR with age by regression analysis in subjects who did not develop any evident disease and who developed contralateral and ispilateral breast cancer (i.e., the disease conditions with the highest number of subjects). The regression of retinol on age was significant. In contrast, the regression of 4-HPR and 4-MPR was not significant even when subjects were divided according to menopausal status. As 4-HPR and 4-MPR were not related with age, subjects were divided into age ranges. Three age ranges were chosen: (a) 45; (b) 46–55; and (c) 56 years. The ranges 45 and 56 years were chosen because they included mostly pre and postmenopausal women, respectively. The range 46–55 years was chosen because it included both pre and postmenopausal women. As regards the regression analysis between retinol and age, when it was performed within each age range, it was significant only in the age range 46–55, which included pre and postmenopausal women. Therefore, in all of the analyses, plasma levels were subdivided according to the three age ranges, also taking into account menopausal status. The levels of 4-HPR, 4-MPR, and retinol were expressed as the mean ± SD. In all analyses, the values were log transformed to approximate a Gaussian distribution. In all statistical analyses, groups with one to three subjects were not considered for comparison, but their means were reported in tables for descriptive purposes.

Retinol levels at baseline were subdivided according to the three age groups, and menopausal status and the differences between the means were evaluated by Student’s t test (Table 2) . The baseline retinol levels were then subdivided according to subsequent disease outcome, and the comparison of each mean versus that of subjects with no evident disease was carried out according to Dunnet’s t test (Fig. 1) . The stability in time of retinol levels in control subjects was evaluated by analyzing the differences between the values at the beginning and end of the intervention period by Student’s paired t test in subjects who had blood drawn at both intervals (Table 3) .

View larger version (45K): [in this window] [in a new window]   Fig. 1. Plasma retinol levels (means ± SD) at baseline according to subsequent disease outcome and toxicity (data referring to fewer than three subjects are not reported). Empty columns, subjects in premenopause; gray columns, subjects in postmenopause. The number of subjects belonging to each group is reported inside the columns. CTR, controls; Cont. or ipsi. ca., contralateral or ipsilateral breast cancer; Met., metastasis; 2nd primary ca., second primary cancer; Tox., toxicity or abnormal laboratory tests. *, P 0.05 versus same age subjects with no evident disease. Dunnet’s t test.

All of the analyses were performed using SAS software (13) . Probability values reported are two sided. Values of P 0.05 were considered significant.

	Results

Top Abstract Introduction Patients and Methods Results Discussion References

 
Subject Characteristics and Pretreatment Plasma Retinol Levels.
The main characteristics of the subjects, whose blood was collected during the 4-HPR breast cancer prevention trial, are described in Table 1 . The two treatment arms were well balanced and comparable with the whole study cohort (1) .

Pretreatment retinol levels of subjects randomized in the 4-HPR and control arms are reported in Table 2 , and they are compared with those of healthy female subjects. Only six subjects aged 45 years were in postmenopause in the 4-HPR (n = 3) and control (n = 3) arms, and only two subjects aged 56 years were in premenopause in the control arm. A comparison between pre and postmenopause was assessed only in the age group 46–55 years. In this age group, postmenopausal subjects had significantly higher retinol levels (P 0.001) than premenopausal subjects. Among premenopausal subjects, retinol levels were lower (P 0.05) in those aged 45 years than in those aged 46–55 years. There were no significant differences in retinol levels between the 4-HPR and control arms. The average retinol levels of subjects participating in the prevention trial were not statistically different from those of healthy female subjects.

To assess the value of retinol levels in predicting disease outcome and toxicity, the baseline retinol levels of subjects in the 4-HPR and control arm were subdivided according to subsequent disease conditions or toxicity and compared with the levels of subjects with no evident disease (Fig. 1) . In the 4-HPR arm, subjects aged 45 years who experienced toxicity during 4-HPR treatment had initial retinol levels significantly lower (P 0.05) than subjects of the same age with no evident disease. In the control arm, baseline retinol levels of the different groups did not differ from those of subjects with no evident disease, except for lower average retinol levels in women in the age group 56 years, who subsequently developed metastasis.

Retinol Plasma Levels of Subjects in the Control Arm during the 5-year Study.
The stability of retinol levels in control subjects during the 5-year study was assessed by comparing retinol levels in subjects who had plasma samples drawn at baseline and at 5 years (Table 3) . There were no changes from 0 to 5 years except for a significant increase in subjects aged 46–55 years who were in premenopause at baseline and had no evident disease.

4-HPR, 4-MPR, and Retinol Plasma Levels during the 5-year Study.
For analysis of samples during 4-HPR intervention, the following criteria of selection were used to obtain consistent data: (a) last drug intake dose, 200 mg as one and not as two separate 100-mg daily doses; (b) blood sampling at 10–18 h from drug intake, i.e., between peak and through concentrations at steady state (4) ; and (c) samples with 4-HPR levels 150 ng/ml, corresponding on the basis of previous kinetics study (14) , to the lower 95% tolerance limit for drug concentration at 18 h. After the selection criteria, 2348 samples from 537 subjects in the 4-HPR arm were assessable for analysis of drug and retinol levels during the 5-year intervention period.

The eventual stability of 4-HPR, 4-MPR, and retinol levels during the intervention period was first assessed. To this aim, regression analysis was performed on 4-HPR, 4-MPR, and retinol levels for each subject with samples drawn at least at three different intervals during treatment. Among the 298 subjects analyzed, the regressions were significant only in very few cases (6% for 4-HPR and 4-MPR and 13% for retinol). The stability of drug and retinol levels was further analyzed by the paired t test in plasma levels of women who had plasma samples drawn at 1 and 5 years (Table 4) . No changes in 4-HPR and 4-MPR plasma levels from 1 to 5 years were found. Retinol levels after the 5-year treatment were slightly lower than the levels at 1 year, and the differences were significant in the groups with no evident disease (P 0.05 and 0.001). In the age group 46–55 years, no differences were found between the means of pre and postmenopausal women at 1 or 5 years. Therefore, all of the following analyses on subjects in the 4-HPR arm were performed, taking into account only the age groups and disease outcome.

Comparison of 4-HPR, 4-MPR, and Retinol Plasma Levels after 1 Year of Treatment.
After the observation of drug and retinol stability during the 5-year treatment, comparison of mean levels for the different age groups according to disease outcomes and toxicity was performed at 1 year, i.e., when more samples were available. The mean levels of 4-HPR, 4-MPR, and retinol of subjects whose plasma was drawn after 1 year of treatment and the mean values of body surface area and BMI at baseline are reported in Table 5 . The proportion of subjects, reported in Table 5 , initially operated on for carcinoma in situ pT1 and pT2 who subsequently developed contralateral or ipsilateral breast cancer and metastasis was similar to that of subjects of the same age with no evident disease (data not shown).

Comparison of plasma levels was first assessed among age groups. In subjects with no evident disease, the 4-HPR and 4-MPR levels of the groups 46–55 and 56 years, which were not different from one another, were significantly higher (P 0.05) than those of the group 45 years, despite concomitant larger body surface areas and BMI (P 0.005). No difference was found among age groups in the other disease conditions.

The plasma levels of subjects with the different disease conditions were then compared with those of subjects with no evident disease. In subjects 45 years, with contralateral or ipsilateral breast cancer, the means of 4-HPR and 4-MPR levels were higher (P 0.05), and the means of retinol levels were lower (P 0.05) than those of subjects of the same age with no evident disease. In subjects of all age groups who developed metastasis, average 4-HPR and 4-MPR levels were higher than in subjects with no evident disease, although the differences were not statistically significant. In these subjects, the SD of 4-MPR levels was also higher. This was attributable to many subjects with abnormally high 4-MPR levels, i.e., 900 ng/ml. Among subjects who developed metastasis, those 56 years had a larger body surface area and higher BMI than subjects with no evident disease of the same age. The few subjects who experienced toxicity had smaller body surface areas (mean values 1.41 and 1.54 m²) than subjects in the other groups (the lowest mean value was 1.59 m² for subjects 45 years with no evident disease), suggesting a proportionally higher drug intake.

The correlations between each pair of variables reported in Table 5 were also assessed. Retinol at baseline, which is not reported in Table 5 , and retinol decrease (i.e., retinol at baseline minus retinol during treatment) were also taken into account. Only subjects with no evident disease and contralateral or ipsilateral breast cancer, i.e., the disease conditions with the highest number of subjects, were considered in the analyses. When drug levels were correlated with body surface area and BMI, significant correlations were found only in subjects 45 years with no evident disease in which 4-HPR levels were inversely associated with body surface area (r = -0.38: P = 0.001) and in subjects 45 years who developed contralateral or ipsilateral breast cancer in which 4-MPR levels were directly associated with BMI (r = 0.61; P = 0.03; data not shown). A highly significant correlation was found between 4-MPR and 4-HPR levels (r 0.59; P 0.03) and between the retinol decrease and retinol levels at baseline (r 0.7; P 0.001) in subjects with no evident disease and in those with contralateral and ipsilateral breast cancer of all age ranges (data not shown). 4-HPR levels were inversely correlated with retinol levels during treatment (r 0.27; P 0.02) in subjects with no evident disease of all age ranges, whereas such a correlation was not found in subjects who developed contralateral or ipsilateral breast cancer (data not shown). As the number of subjects with no evident disease was larger than that of subjects with contralateral or ipsilateral breast cancer, for a more adequate comparison, the same correlation was also assessed on a number of subjects with no evident disease (randomly selected) equal, for each age range, to that of subjects with contralateral and ipsilateral breast cancer. The correlation between 4-HPR levels and retinol levels during treatment was still significant (r 0.48; P 0.05; data not shown).

	Discussion

Top Abstract Introduction Patients and Methods Results Discussion References

 
The primary objectives of the study were to assess, in subjects participating in a 4-HPR prevention trial, the influence of age and menopausal status on drug and retinol plasma levels and prospectively evaluate their association with a second breast malignancy.

At randomization, the 4-HPR and control arms had comparable retinol levels. As reported previously by other authors (15 , 16) , we found a positive relation between age and retinol levels. We also found that retinol levels are affected by menopausal status. Among women of the same age range, those in postmenopause had higher retinol levels than those in premenopause. In addition, among women in the control arm, only those aged 46–55 years who were in premenopause at baseline showed, during the 5-year trial, a significant increase in retinol levels, which was presumably caused by the change in menopausal status. The reasons for the observed increase in women with age and after menopause are not known. Several reports indicate that retinol levels are variously associated with serum cholesterol and triglycerides (17 , 18) . The increase in retinol levels found in older women might be linked to the increase in circulating lipoproteins that occurs with aging. The results of the few studies that have explored the influence of sex hormones on retinol plasma levels do not clarify the issue. In fact, oral contraceptive therapy in young women has been found to induce a significant increase in retinol levels (19, 20, 21) . Although the reasons for the observed difference are not known, the findings indicate that age and menopausal status should always be taken into account when interpreting retinol levels in women.

Evidence from our and previous studies (6 , 8) suggests that retinol levels are not associated with a risk of breast cancer. Our results on the role of retinol levels as predictive of breast tumor recurrence indicate that, in women operated on for stage I breast cancer, retinol levels have no prognostic value for contralateral or ipsilateral breast cancer. Less conclusive are the results on the role of retinol levels in predicting breast cancer metastasis. Control subjects >56 years who subsequently developed metastasis had lower retinol levels than disease-free subjects. However, such a difference was not found in subjects treated with 4-HPR. Additional studies are necessary to clarify this issue.

Estimates of drug plasma levels demonstrated that a daily p.o. dose of 200 mg of 4-HPR resulted, at 10–18 h after administration, in 4-HPR and 4-MPR plasma levels of 400 ng/ml, corresponding to 1 µM. The 4-HPR concentrations found effective in suppressing the in vitro growth of tumor cells range from 1 to 10 µM (22) . Therefore, plasma levels of 1 µM 4-HPR correspond to the least effective concentrations in in vitro models. However, we showed previously that 4-HPR accumulates in the breast because its concentrations in nipple discharge were 10 times higher than those in plasma (4) . 4-HPR and 4-MPR levels, which were directly related, remained constant during the 5-year treatment. The results confirm previously reported data found in a small group of women participating in a Phase I trail (4) .

With regard to the possible influence of age and menopausal status on 4-HPR pharmacokinetics, the present data indicate that circulating 4-HPR and 4-MPR levels are not linked to menopausal status but that they are influenced by patient age. After identical daily doses during 1 year of treatment, subjects 45 years had slightly, but significantly, lower 4-HPR and 4-MPR plasma levels than the older subjects. This occurred despite the marked lower body surface area of women 45 years than those in the other age ranges. Lower drug absorption, higher metabolism to undetected metabolites, or higher biliary excretion might account for the lower 4-HPR and 4-MPR levels found in the youngest women. After their absorption from the gastrointestinal tract, retinoids, which are water insoluble compounds, bind to serum albumin and lipoproteins and are transported to the tissues. Although acidic retinoids, like all-trans retinoic acid, bind preferentially to albumin, neutral retinoids bind to lipoproteins (23) . We do not know how 4-HPR is transported in plasma, but because 4-HPR is a neutral retinoid, it should be carried by lipoproteins. Therefore, the increased plasma levels of 4-HPR in older subjects might be attributable to the drug binding to concurrent plasma lipoproteins, whose levels usually increase with increasing age.

Unexpectedly, we found that subjects 45 years with breast cancer recurrence had slightly, but significantly, higher drug levels than subjects with no evident disease. Unfortunately, because the sample size in the two groups was unbalanced and the difference was small, we cannot draw conclusions on the role of drug plasma levels as predictive of 4-HPR efficacy. However, the results, in conjunction with the finding of higher drug plasma levels in older subjects who did not show any preventive benefit from 4-HPR treatment (1) , suggest an inverse association between plasma drug levels and 4-HPR preventive effects. An explanation for this intriguing result might be that higher drug plasma levels reflect lower drug concentrations in the tissues where they are needed. It may be that the binding of 4-HPR to lipoproteins in older women and young nonresponding women might inhibit entry of the drug into cells. In vitro data on tumor cell lines support such a hypothesis. In in vitro assays, the addition of retinoids using serum-free conditions or low serum concentrations resulted in dose-dependent growth inhibitory effects, which decreased when serum or serum components were added (24, 25, 26) . It has also been demonstrated that reduced growth inhibitory effects were associated with decreased retinoid uptake by the cells (25) . The same applies to the in vitro growth inhibitory effects of 4-HPR.⁴

Although the difference was not statistically significant, subjects who subsequently developed metastases also had higher 4-HPR and 4-MPR levels than subjects with no evident disease. Moreover, a high percentage of these subjects had abnormally high (900 ng/ml) 4-MPR plasma levels. 4-HPR and 4-MPR are both lipophilic, and 4-MPR has a longer storage than 4-HPR in deep tissue compartments, presumably fat, from which it is slowly released (4) . The abnormally high 4-MPR concentrations found in subjects who subsequently developed metastasis presumably reflect a high percentage of adipose tissue in these subjects.

The results of the 4-HPR breast tumor prevention trial have shown the good tolerability of the retinoid at 200 mg/day over a 5-year treatment (1 , 12) . The present results indicate that the few subjects who experienced 4-HPR toxicity and whose mean drug plasma levels are herein reported had a smaller body surface area than subjects who showed no toxicity. The data suggest that 4-HPR should be administered on the basis of body surface area. Moreover, 4-HPR toxicity was associated with low retinol levels before 4-HPR administration but only in subjects aged 45 years. This age group had the lowest pretreatment retinol levels, and the additional reduction caused by 4-HPR in these subjects may have resulted in retinol levels below threshold limits.

Regarding the effect of 4-HPR on retinol plasma levels, we had shown previously that 4-HPR reversibly reduces the plasma concentrations of retinol and of its transport protein, RBP (4 , 5) . We also showed that the high binding affinity of 4-HPR for RBP and the lack of binding of the complex 4-HPR-RBP to transthyretin (27) might account for the reduction of retinol secretion from retinol-secreting organs. Retinol levels after a 5-year treatment were always slightly, but significantly, lower than those found at 1 year. The difference, although it does not seem to be biologically relevant, might indicate 4-HPR accumulation in retinol-secreting organs like the liver. A new finding was that the reduction in retinol levels was strongly and directly correlated with pretreatment retinol levels. Therefore, pretreatment retinol levels may predict retinol level reduction by 4-HPR; in fact, the higher the initial values, the higher the absolute decrease, with the percentage decrease remaining the same. Another interesting observation was that the inverse correlation between 4-HPR and retinol levels during treatment was significant in subjects with no evident disease, whereas it was not significant in those in whom breast cancer recurred. This result seems to further support the evidence of differences in 4-HPR pharmacokinetics between subjects with no evident disease and those who did not benefit from 4-HPR treatment. Interestingly, differences in retinoid metabolism have been found between human tumors and the respective normal tissues (28) .

In conclusion, in a prospective study in women participating in a breast tumor prevention trial with 4-HPR, we found that subjects 45 years had lower drug plasma levels than older subjects, and, among young subjects, those with breast cancer recurrence had higher drug levels. A tentative explanation for this unexpected finding could be related to drug interaction with serum proteins, drug sequestration in plasma, and consequent interference with the tumor preventive potential. The hypothesis of serum components as determinant of 4-HPR plasma levels and bioavailability should be investigated in future studies with the retinoid.

	Acknowledgments

 
We thank Dr. Carmen Pollini for her help in data analysis and critical discussion of the results and Laura Zanesi for secretarial assistance.

	Footnotes

 
The costs of publication of this article were defrayed in part by the payment of page charges. This article must therefore be hereby marked advertisement in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.

¹ Supported by NIH/National Cancer Institute Grants CA38567 and CA72286 and the Associazione Italiana per la Ricerca sul Cancro.

² To whom requests for reprints should be addressed, at Istituto Nazionale Tumori, Via Venezian 1, 20133 Milan, Italy. Phone: 39-02-23902706; Fax: 39-02-23902692; E-mail: franca.formelli{at}istitutotumori.mi.it

³ The abbreviations used are: 4-HPR, fenretinide; 4-MPR, N-(L-methoxyphenyl)retinamide; BMI, body mass index; RBP, retinol binding protein.

⁴ Formelli et al., manuscript in preparation.

Received 6/17/02; revised 9/18/02; accepted 10/10/02.

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Top Abstract Introduction Patients and Methods Results Discussion References

 

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