Endogenous Natriuretic Factors 7: Biospecificity of a Natriuretic gamma -Tocopherol Metabolite LLU-alpha

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Vol. 282, Issue 2, 657-662, 1997

Endogenous Natriuretic Factors 7: Biospecificity of a Natriuretic $gamma$ -Tocopherol Metabolite LLU- $alpha$ ¹

E. David Murray, Jr., William J. Wechter, Darko Kantoci, Wen-Hui Wang, Tim Pham, David D. Quiggle, Karina M. Gibson, Douglas Leipold and Beatrice M. Anner

Laboratory of Chemical Endocrinology, Loma Linda University School of Medicine, Loma Linda, California (E.D.M. Jr., W.J.W., D.K., T.P., D.D.Q., K.M.G., D.L.), Department of Pharmacology, New York Medical College, Valhalla, New York (W.-H.W.) and Department of Pharmacology, Geneva University School of Medicine, Geneva, Switzerland (B.M.A.)

	Abstract

Top Abstract Introduction Methods Results Discussion References

The structural elucidation and mechanism of action of a potential component, LLU- $alpha$ , of what is possibly a multifactorial complexknown as "natriuretic hormone" was recently reported [Wechter,W.J. et al. (1996a) Proc. Natl. Acad. Sci. U.S.A. 93: 6002-6007]."Natriuretic hormone," a long-sought factor, is believed to regulateextracellular fluid volume and consequently be pathomimetic forhypertension, cirrhosis, congestive heart failure and other volumeexpanded states. The studies reported herein further characterizeLLU- $alpha$ . The precursor of the endogenous LLU- $alpha$ was demonstratedto be $gamma$ -tocopherol by radiolabeling studies. The pharmacokineticsof infused rac-LLU- $alpha$ proved to be biphasic (half-lives: 12 minand 6 h). Specificity of the inhibition of the 70 pS potassiumchannel of the thick ascending limb of the loop of Henle was examinedwith the natural S-enantiomer being the most potent known inhibitorwhereas the analogous $alpha$ -tocopherol metabolite, rac-5-Me-LLU- $alpha$ ,showed no inhibition. Rac-LLU- $alpha$ does not inhibit two isozymesof the Na⁺/K⁺-ATPase. LLU- $alpha$ is natriuretic acting via inhibition of the 70pS potassium channel and not Na⁺/K⁺-ATPase, the assumed mechanism of action of the "natriuretic hormone."LLU- $alpha$ , a metabolite of a vitamin, if it were found to play a rolein the regulation of extracellular fluid volume, would be thesecond example of a vitamin acting as a precursor for a hormone.Of considerable interest is the fact that this manuscript reportsthe first biological activity of $gamma$ -tocopherol, a member of thevitamin E complex.

	Introduction

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"Natriuretic hormone," the putative controller of extracellular fluid volume (de Wardener et al., 1961) has been sought formore than 30 years. This compound was believed to be responsiblefor the three effects observed during saline-induced volume expansion:prolonged natriuresis, inhibition of sodium transport and increasedvasoreactivity. Most search paradigms have focused on the inhibitionof sodium transport, specifically inhibition of the Na⁺/K⁺-ATPase (sodium pump) or immunocross-reactivity to antibodiesdeveloped to the pump inhibitors ouabain or digoxin, as an assayto detect this compound during isolation (Wechter and Benaksas,1990; Benaksas et al., 1995). This has led to the isolation ofdigoxin (Goto et al., 1990) and "iso-ouabain" (Ludens et al.,1991; Mathews et al., 1991; Tymiak et al., 1993; Zhao et al.,1995). Digoxin and ouabain, however, are kaliuretic and not natriuretic(Crabos et al., 1987; Murray et al., 1995; Pamnani et al., 1991;Smyth et al., 1992; Sekihara and Yuzaki, 1993). Therefore, thissearch tool is inappropriate except for bufalin-like compoundswhich are natriuretic (Pamnani et al., 1991). Our search has concentratedon the natriuresis attributed to this putative hormone, resultingin detection of several natriuretic components in human uremicurine (Benaksas et al., 1993; Murray et al., 1995).

The isolation, purification and structure determination of the most interesting of these compounds to date, LLU- $alpha$ , has beendescribed (Wechter et al., 1996a). A probable metabolite of $gamma$ -tocopherol,LLU- $alpha$ , was shown to be natriuretic, an inhibitor of the 70 pSATP-sensitive K⁺ (K_ATP) channel in the TAL and without an effect on hemodynamicsas measured by the glomerular filtration rate (Wechter et al.,1996a). It was also demonstrated not to be an inhibitor of theNa⁺/K⁺-ATPase in MDBK cells. Unlike atrial natriuretic peptide, whichis also not an inhibitor of the sodium pump (Chiou and Vesely,1995; Charlton and Baylis, 1990), LLU- $alpha$ exhibits a prolonged natriuresislike that described for "natriuretic hormone" (de Wardener etal., 1961).

In the present study LLU- $alpha$ is further characterized. Its origin from $gamma$ -tocopherol is established. The pharmacokinetics ofintravenously infused LLU- $alpha$ is reported and compared with thetime course of natriuresis. The specificity of the inhibitionof the 70 pS K⁺ channel by the enantiomers of LLU- $alpha$ is determined. The analogous $alpha$ -tocopherol metabolite is also investigated for its ability toinhibit this potassium channel. The inhibition of the Na⁺/K⁺-ATPase from different sources is tested.

	Methods

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LLU- $alpha$ and derivatives. The compounds used in these studies (fig. 1) were synthesized as described by Kantoci et al. (accompanying paper, 1997). Theenantiomers of LLU- $alpha$ were purified by preparative chiral HPLCas described by Kantoci et al. (accompanying paper, 1997).

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Fig. 1. Compounds used in these studies. S-LLU- $alpha$ is the natural enantiomer (Kantoci et al., accompanying paper, 1997).

Metabolism of $gamma$ -tocopherol in rats. Two rats (Sprague-Dawley, Harlan) were each injected intraperitoneally with 500 µCi/kg of [³H]- $gamma$ -tocopherol (9.6 Ci/mmol, Amersham custom synthesis) in 2.5ml/kg of 10% ethanol in corn oil (Chiku et al., 1984; Simon etal., 1956a, b). The rats were then placed into metabolic cagesfor urine collection for 4 days. The urine (220 ml) was pooled,solids removed by filtration. The solution was extracted with2 g Amberlite XAD-2 (Aldrich, Milwaukee, WI) with stirring for18 h. The XAD was recovered by filtration and extracted with 4volumes of methanol totaling 60 ml. The methanol was removed undera stream of 5.0 µm filtered air. The dried residue was resuspendedin 1.8 ml of 40:60 methanol/0.2 M acetic acid for chromatography.Beckman System Gold (126 pump, 168 diode array detector) controlledby System Gold software v 5.1 on PC was used for all chromatography.A C₁₈ RP-HPLC (Beckman Ultrasphere ODS column; 5 µm; 10 × 250mm) was eluted at 2 ml/min with a gradient of 0.2 M acetic acid(A), methanol (B) and 70% toluene/30% methanol (C) (60% A:40%B for 5 min, a linear gradient to 50% A:50% B over 5 min, a lineargradient to 30% A:70% B over 55 min, a linear gradient to 100%B over 2 min, 100% B for 3 min, 100% C for 8 min, 100% B for 7min). The eluant was monitored for absorbance at 265 and 290 nmand ultraviolet spectra were collected (202-390 nm). Seventy-eightfractions of 1-min duration were collected. An aliquot (50 µl)of each fraction was counted in 5 ml of liquid scintillation cocktail(ScintiVerse^TM Bio-HP, Fisher, Tustin, CA) in a LS 3801 LiquidScintillation Counter (Beckman, San Ramon, CA). Fractions (39-42)eluting in the region known to contain LLU- $alpha$ were pooled, 25 µgof synthetic, racemic LLU- $alpha$ was added and the pooled materialwas dried under reduced pressure in a centrifugal vacuum concentrator(Jouan, Winchester, VA). The residue was dissolved in 1.8 ml of15:85 45 mM acetic acid in acetonitrile/50 mM acetic acid (aq.)and chromatographed on C₁₈ RP-HPLC (Beckman Ultrasphere ODS column;5 µm; 4.6 × 250 mm) eluted at 1 ml/min with a gradient of 50 mMacetic acid (A) and 45 mM acetic acid in acetonitrile (B) (85%A:15% B for 3 min, a linear gradient to 100% B over 42 min, 100%B for 5 min). The eluant was monitored for absorbance at 265 and295 nm by the diode array detector. Fifty 1-min fractions werecollected with aliquots (100 µl) counted as described above. Thisexperiment was performed in duplicate.

In vivo bioassay. The assay for natriuresis in conscious rats has previously been described in detail (Benaksas et al., 1993), but will be brieflyreiterated here. The bladder of ether-anesthetized female Sprague-Dawley(Harlan) rats (200-250 g) was catheterized for collection of urinein 10-min periods. The femoral artery and vein were cannulatedfor monitoring of mean arterial pressure and infusion of saline(0.49 ml/h) and samples, respectively. After recovery from anesthesia,furosemide (100 µg, approximately 0.4 mg/kg b.wt.; 1 mg/ml in0.17% saline) was infused as a positive control at the beginningof the sixth 10-min urine collection period. The sample was infusedat the beginning of the 17th 10-min period. Urine was collectedfor another 150 min. The volume of the urine was determined gravimetrically.The urine Na⁺ and K⁺ concentrations were determined with a Beckman E2A electrolyteanalyzer. From these data the sodium excretion values (UNaV; [UNaV= urine sodium concentration × urine volume per time]) were calculated.

The net sodium excretion for the infusion of furosemide or sample was calculated as follows. The median (or middle) sodiumexcretion value (µmoles Na⁺/10-min period) for the five periods before infusion of furosemideor sample was used to establish a baseline value for the calculationof $Delta$ UNaV (= µmoles Na⁺ in a 10-min period $-$ base-line µmoles Na⁺) for the administration of either furosemide or sample, respectively.The sum of $Delta$ UNaV for the four periods after infusion of furosemidewas the net sodium excreted for furosemide, defined as furosemideresponse (FR). The sum of $Delta$ UNaV for the 15 periods (150 min) afterinfusion of the sample was the net sodium excreted for the sample,defined as sample response (SR). The natriuretic response of asample was then normalized to the natriuretic response of thedose of furosemide infused. This natriuretic ratio (R_N) (or normalizednatriuretic response) of a sample was calculated by dividing SRby FR (R_N = SR/FR). A sample is considered natriuretically activeif R_N $>=$ .55 (greater than 99% confidence limits).

Pharmacokinetics of LLU- $alpha$ . The in vivo bioassay for natriuresis (described above) was adapted for these experiments. At the time of sample infusion,10 µg of [³H]LLU- $alpha$ (4.2 µCi/nmol, Amersham Custom Synthesis, 0.25 mCi/mlethanol; 640 µl dried under a stream of argon and resuspendedin 100 µl of 47.5% ethanol) was infused, and the saline infusionrate was changed to 1 ml/min. The experiment was performed ontwo animals. Blood (approximately 0.5 ml) was drawn from eachanimal into heparinized microfuge tubes at various time points.Blood was drawn from animal 1 at 1, 5, 30 and 120 min and fromanimal 2 at 2, 15, 60 and 240 min. The blood was centrifuged for5 min. An aliquot of plasma (100 µl) was withdrawn and placedinto a 15-ml centrifuge tube. HCl (2 N, 20 µl) was added to eachcentrifuge tube and vortexed for 30 sec. Hexane/ether (4:1, 2ml) was added to each tube and the tube was vortexed for 3 min.The samples were sonicated and centrifuged as necessary and 1.5ml of the hexane/ether sample was removed and placed in a glasstest tube. Unlabeled synthetic, racemic LLU- $alpha$ (50 µg) was addedto each sample. The solvent was removed under a stream of filteredair. The sample was resuspended in 1.8 ml of 15:85 45 mM aceticacid in methanol/50 mM acetic acid (aq.) and chromatographed onacetic acid/acetonitrile RP-HPLC as described in "Metabolism of $gamma$ -Tocopherol in Rats." Fifty 1-min fractions were collected, withaliquots (100 µl) counted as above. A pilot study was conductedusing one animal infused with 10 µg of [³H]LLU- $alpha$ and blood drawn at 5, 15, 30, 60 and 160 min.

Na⁺/K⁺-ATPase inhibition assays. Inhibition of the Na⁺/K⁺-ATPase by the reduction of ⁸⁶Rb⁺ uptake into human lymphocytes was examined. Lymphocytes were isolatedfrom heparinized blood with a Histopaque-1077 (Sigma, Buchs, Switzerland)density gradient and then washed with buffer by centrifugationsimilar to previously described methods (Anner et al., 1994).Cell viability was examined by the trypan blue dye exclusion testand was found to be greater than 99%. Lymphocytes (5 × 10⁶ cells) were incubated in the presence or absence of synthetic,racemic LLU- $alpha$ (125 µM, final concentration) in 50 µl of PBS (154mM NaCl, 10 mM sodium phosphate, pH 7.2-7.4) with 50 nCi ⁸⁶Rb⁺ for 30 min at 36°C with shaking. Cells were washed three timeswith PBS (once) or D-PBS (twice; 137 mM NaCl, 2.68 mM KCl, 0.90mM CaCl₂, 0.49 mM MgCl₂, 6.46 mM Na₂HPO₄, 1.47 mM KH₂PO₄) by centrifugationat 0°C at 500 × g. The recovered cells were then counted. Cellviability was checked by trypan blue dye exclusion after incubationunder the same conditions but without ⁸⁶Rb⁺. Na⁺/K⁺-ATPase was isolated from lamb renal outer medulla as describedpreviously (Anner et al., 1992). Na⁺/K⁺-ATPase activity was measured by the linked enzyme assay methoddescribed (Anner et al., 1992). Synthetic, racemic LLU- $alpha$ in 50mM sodium phosphate buffer, pH 7.2, was added to a final concentrationof 125 µM either during the assay or 30 min. before the assayfor preincubation at 37°C. Only buffer was added for control assays.

Patch-clamp experiments. Pathogen-free Sprague-Dawley rats (male or female, 80-120 g) were maintained on normal rat chow before being sacrificed asdescribed previously (Wang, 1994). Kidneys were then removed andthin (1 mm) coronal sections were cut. The cortical and medullaryTAL tubules were dissected at room temperature. The TAL tubuleswere immobilized onto cover glass coated with Cell-Tak (CollaborativeResearch, Bedford, MA). The cover glass was then placed in a chambermounted on an inverted microscope and the tubules superfused at37°C with Hepes-buffered Ringer's solution (135 mM NaCl, 5 mMKCl, 1.5 mM MgCl₂, 1.8 mM CaCl₂, 5 mM glucose, 10 mM Hepes, pH7.4). The apical membrane was exposed by cutting the tubule witha sharpened micropipette. Single-channel currents were recordedin cell-attached, inside-out configuration with 140 mM KCl inthe pipette with a resistance of approximately 4 to 6 megohm.The recordings were collected with an Axon 200A patch-clamp amplifier.Single-channel currents were low-pass filtered at 1 kHz with aneight-pole Bessel filter (Frequency Devices 902LPF) and convertedto digitized signals at a sampling rate of 44 kHz by a Sony PCM-501ESpulse code modulator and a videotape recorder. Analysis was donewith use of the pCLAMP software (v. 6.0, Axon Instruments, Burlingame,CA) on an IBM-compatible 486 computer. The potency of the inhibitionof the K⁺ channel is expressed as IC₅₀, which was calculated by linearregression analysis.

	Results

Top Abstract Introduction Methods Results Discussion References

70 pS K⁺ channel inhibition. Racemic, synthetic LLU- $alpha$ has been previously shown to inhibit the 70 pS K⁺ channel in the TAL of the loop of Henle with an IC₅₀ of 6 nM(Wechter et al., 1996a and fig. 2). R- and S-LLU- $alpha$ as well asracemic, synthetic 5-methyl-LLU- $alpha$ (the analogous metabolite of $alpha$ -tocopherol) were tested in this system. 5-Methyl-LLU- $alpha$ demonstratedno inhibition of the 70 pS K⁺ channel in the concentration range of 100 to 500 nM (fig. 2),whereas S-LLU- $alpha$ (IC₅₀ = 3 nM) was a more potent inhibitor thanthe racemate and R-LLU- $alpha$ was about 20-fold less effective, IC₅₀= 51 nM (fig. 2).

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Fig. 2. Inhibition of the 70 pS K⁺ channels from TAL. S-enantiomer of rac-LLU- $alpha$ (closed squares), R-enantiomer of rac-LLU- $alpha$ (closedtriangles), rac-LLU- $alpha$ (closed circles) and rac-5-methyl-LLU- $alpha$ (open circles) were examined for their ability to inhibit thepotassium channel as described under "Methods." Data are presentedas mean ± S.E.M.

Isolation of [³H]LLU- $alpha$ from [³H] $gamma$ -tocopherol-treated rats. To test the hypothesis that LLU- $alpha$ originates as a result of side-chain degradation of $gamma$ -tocopherol, rats were administered[³H] $gamma$ -tocopherol. Urine collected from these rats was extractedand chromatographed as described under "Methods." The final chromatographicstep is shown in figure 3. A peak of radioactivity (3800 cpm total)coelutes with added nonlabeled, synthetic racemic LLU- $alpha$ standard.The approximate overall yield from administered [³H] $gamma$ -tocopherol was 2 × 10³%.

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Fig. 3. Last step in isolation of [³H]LLU- $alpha$ from [³H] $gamma$ -tocopherol-treated rats. Absorbance at 295 nm of eluant collected from the aceticacid/acetonitrile chromatography of urine from rats administered[³H] $gamma$ -tocopherol is shown (solid line). The programmed acetonitrilegradient is plotted (- - -). Total cpm in each fraction (correctedfor background cpm) is represented by the open bars. The arrowindicates the elution time of the synthetic, racemic LLU- $alpha$ standard.

Pharmacokinetics of LLU- $alpha$ . [³H]LLU- $alpha$ infused intravenously demonstrates biphasic pharmacokinetics (fig. 4). The data were fit to the equation:

y=a ∗ e(−<IT>k1∗t</IT>)<IT>+b ∗ e</IT>(−<IT>k2∗t</IT>)

and the data were weighted (1/y [cpm]). The half-life for the first phase is 12.5 min. whereas that for the second phaseis 6.3 h. Complete clearance is estimated to be 3 days.²

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Fig. 4. Natriuretic/diuretic response and pharmacokinetics of LLU- $alpha$ . Sodium excretion (UNaV, solid bars) and water excretion (UV,open bars) as a result of infusion of 10 µg synthetic, racemicLLU- $alpha$ are measured for 150 min. The five 10-min periods beforeinfusion were used to determine the background excretions. R_N= .54 for this experiment. (Inset) Levels of [³H]LLU- $alpha$ in 100 µl plasma determined by extraction and RP-HPLCas described under "Methods." Each point represents a single determination.

Inhibition of Na⁺/K⁺-ATPase. Inhibition of the Na⁺/K⁺-ATPase by synthetic, racemic LLU- $alpha$ was examined with two different methodologies. Synthetic, racemicLLU- $alpha$ did not reduce uptake of ⁸⁶Rb⁺ into human lymphocytes at 125 µM (data not shown). Isolated Na⁺/K⁺-ATPase, from lamb renal outer medulla, examined by a linked enzymeassay was not inhibited by 125 µM synthetic, racemic LLU- $alpha$ (datanot shown).

	Discussion

Top Abstract Introduction Methods Results Discussion References

Biology of LLU- $alpha$ . We previously showed that synthetic, racemic LLU- $alpha$ does not inhibit the sodium pump in MDBK cells (Wechter et al., 1996a).In the present study we demonstrate that it also does not inhibitthe Na⁺/K⁺-ATPase in lymphocytes nor from renal outer medulla (data notshown). Thus LLU- $alpha$ does not inhibit the $alpha$ ₁ (present in the threesources tested [Anner et al., 1992; Vereninov et al., 1993]) and $alpha$ ₃ (present in outer medulla [Barlet-Bas et al., 1993]) isoformsof the sodium pump. This lends additional support to the hypothesisthat sodium pump inhibition is a poor search tool for isolationof natriuretic substances with the exception of bufalin-like compounds(Wechter and Benaksas, 1990; Benaksas et al., 1995; Pamnani etal., 1991). This is the second compound isolated and characterizedby our laboratory that is natriuretic but is not a sodium pumpinhibitor (Wechter et al., 1996b), and other compounds that fitthis description are yet to be characterized (Benaksas et al.,1993; Murray et al., 1995). The compounds isolated by Na⁺/K⁺-ATPase inhibition as a search tool, digoxin (Goto et al., 1990)and iso-ouabain (Ludens et al., 1991; Matthews et al., 1991; Tymiaket al., 1993; Zhao et al., 1995), may have a role in volume orblood pressure homeostasis; however, we believe this functionis not likely to occur via natriuresis (Pamnani et al., 1991;Sekihara and Yuzaki, 1993; Wechter and Benaksas, 1990; Benaksaset al., 1995).

The pharmacokinetics of LLU- $alpha$ involves two distinct phases (fig. 4). The early phase with a t_1/2 of 12.5 min is probably notcritical to the chronic natriuretic activity. There is an indication,however, that a very short-lived diuresis correlates with theseearly higher levels of S-LLU- $alpha$ . The longer t_1/2 (6.3 h) appearsto correlate with the chronic activity that exhibits a high correspondenceof natriuresis and diuresis. The 6-h t_1/2 is indicative of a secondcompartment which may be serum albumin or it may represent a reservoirsuch as the kidney, because compounds of this class (organic acids)are generally excluded from the central nervous system, anotherpotential site of action. We plan to study intrathecal administrationand albumin binding of LLU- $alpha$ .

The lactone of the oxidation product of synthetic rac-LLU- $alpha$ (fig. 1) was assayed in the rat by the in vivo bioassay for natriuresisover the range of 0.04 to 400 µg/kg and was not natriuretic norvasoactive (data not shown). Synthetic, racemic LLU- $alpha$ had beenshown previously not to affect mean arterial pressure in thisassay (Wechter et al., 1996a

). Another inhibitor of the 70 pSK⁺ channel, 20-hydroxy-eicosatetraenoic acid (Wang and Lu, 1995

),does however demonstrate vasoactivity in the spontaneously hypertensiverat (Schwartzman and McGiff, 1995

). The vasoactivity of LLU- $alpha$ therefore needs to be examined in other systems. Once synthesized,the hydroquinone of the lactone of the oxidation product of LLU- $alpha$ will be examined for natriuresis and vasoactivity.

In previous studies, the effect of synthetic, racemic LLU- $alpha$ on the 70 pS K_ATP channel in the TAL cells was investigated asa potential mechanism of natriuresis (Wechter et al., 1996a

).Inhibition of this channel in the TAL leads to natriuresis bypreventing potassium recycling for the Na⁺/K⁺/2Cl cotransporter (Greger, 1985

; Hebert and Andreoli, 1984

; Gregerand Schlatter, 1981

). In the current study the individual enantiomersof LLU- $alpha$ were examined in patch-clamp experiments. The S-enantiomerof LLU- $alpha$ (the naturally occurring enantiomer; Kantoci et al.,accompanying paper, 1997) proved to be an even more potent inhibitorof the 70 pS K⁺channel than the racemate (fig. 2). The R-enantiomer, however,although not devoid of activity was about 20-fold less potent(fig. 2) than the S-enantiomer. Significantly, the analogous compoundderived from $alpha$ -tocopherol (5-Me-LLU- $alpha$ ; Schönfeld et al., 1993

;Schultz et al., 1995

) was completely inactive as a potassium channelinhibitor at the concentrations tested (100-500 nM; fig. 2). Theseresults indicate great structural specificity to the biology ofLLU- $alpha$ and its binding to the 70 pS K⁺ channel. The addition of a single methyl group being biologicallysignificant is not unusual (e.g., methylated steroids).

The interesting observation is that a metabolite of a minor component of the Vitamin E complex, obtained only through diet,is an effector of the 70 pS K⁺channel. In recent studies in which 5-Me-LLU- $alpha$ was isolated fromhuman urine, the urine donors were given relatively large dosesof $alpha$ -tocopherol (650 mg/day and greater; Schultz et al., 1995

;Schönfeld et al., 1993

). 5-Me-LLU- $alpha$ was not detected in any ofthe pools of urine from which LLU- $alpha$ was isolated. It may be that5-Me-LLU- $alpha$ was present as a conjugate. In those studies in which5-Me-LLU- $alpha$ was isolated (Schultz et al., 1995

; Schönfeld et al.,1993

), the investigators questioned the role played by VitaminE ( $alpha$ -tocopherol) as an antioxidant, because the major isolatedmetabolite was not the oxidized Simon's metabolites (Simon etal., 1956

a, b). The antioxidant potential of an $alpha$ -tocopherol,however, is greater than that of $gamma$ -tocopherol (reviewed by Kamal-Eldinand Appelqvist, 1996

), which thus increases the likelihood ofthe chroman ring of $gamma$ -tocopherol remaining intact. At least for $gamma$ -tocopherol the proposed side-chain oxidation without the chromanring oxidation metabolic pathway may be necessary for the productionof an important regulator of the 70 pS K_ATP channel and possiblyin the regulation of extracellular fluid volume.

Production of LLU- $alpha$ from $gamma$ -tocopherol. When LLU- $alpha$ was first identified it was assumed that it originated from metabolism of $gamma$ -tocopherol, most likely by side-chainoxidation. In this study it is demonstrated that [³H]-LLU- $alpha$ can be obtained from urine of rats administered [³H] $gamma$ -tocopherol, thus providing evidence that LLU- $alpha$ is a metaboliteof $gamma$ -tocopherol. This is in agreement with previous studies of $alpha$ -tocopherol in humans and $delta$ -tocopherol in rats (Chiku et al.,1984; Schönfeld et al., 1993; Schultz et al., 1995). That LLU- $alpha$ originates from side-chain degradation without oxidation of thechroman ring is confirmed by the study of Kantoci et al. (accompanyingpaper, 1997) demonstrating that the stereochemistry at C-2 isS or the same configuration as that of the parent $gamma$ -tocopherol(Burton and Ingold, 1989).

We currently have a study underway to determine the concentration of S-LLU- $alpha$ in the urine of pregnant women, congestive heartfailure, cirrhosis, uremic and head trauma patients to determinethe relationship between S-LLU- $alpha$ levels and volume-expanded states.If there is a correlation present, then the multifactorial controlof extracellular volume including $gamma$ -tocopherol might prove tobe analogous to that of vitamin D being a precursor to a hormone.The possibility of $gamma$ -tocopherol acting as a precursor to a hormonewould imply the need for regulation of production of S-LLU- $alpha$ viastorage, metabolism and other processes. This will undoubtedlyprove a very interesting area for future studies. The discoveryof LLU- $alpha$ is also the first time that a biological activity hasbeen reported for $gamma$ -tocopherol.

	Acknowledgments

We acknowledge the excellent technical assistance of M. Moosmayer (Geneva) in performing the Na⁺/K⁺-ATPase measurements.

	Footnotes

Accepted for publication April 8, 1997.

Received for publication December 6, 1996.

¹ This work was supported by Adventist Health Systems/Loma Linda (E.D.M., D.K., W.J.W.) and the National Institutes of Health(W.-H.W; grants DK 47402 and HL 34300) and Swiss National ScienceFoundation (B.M.A.; grant 31-37-552.93).

² The kinetic constants are: k₁ = 5.56 × 10² min¹; a = 118,000 cpm; k₂ = 1.82 × 10³ min¹; and b = 26,900 cpm. From the single-animal pilot experimentthe first-phase half-life is 10.9 min and the second-phase half-lifeis 6 h in close agreement with the reported experiment.

Send reprint requests to: William J. Wechter, Ph.D., FCP, Laboratory of Chemical Endocrinology, Room 1512, Department of Medicine, School of Medicine, Loma Linda University, Loma Linda, CA 92350.

	Abbreviations

TAL, thick ascending limb; MDBK, Madin-Darby bovine kidney; HPLC, high-performance liquid chromatography; 5-Me-LLU- $alpha$ , 5-methyl-LLU- $alpha$ ; PBS, phosphate-buffered saline; Hepes, 4-(2-hydroxyethyl)-1-piperazineethanesulfonic acid.

	References

Top Abstract Introduction Methods Results Discussion References

Anner, B. M., Moosmayer, M. and Imesch, E.: Mercury blocks Na-K-ATPase by a ligand-dependent and reversible mechanism. Am. J. Physiol. 262: F830-F836, 1992[Abstract/Free Full Text].
Anner, B. M., Lacotte, D., Anner, R. M. and Moosmayer, M.: Interaction of hypothalamic Na, K-ATPase inhibitor with isolated human peripheral blood mononuclear cells. Biosci. Rep. 14: 231-242, 1994[Medline].
Barlet-Bas, C., Arystarkhova, E., Cheval, L., Marsy, S., Sweadner, K., Modyanov, N. and Doucet, A.: Are there several isoforms of Na, K-ATPases alpha subunit in the rabbit kidney? J. Biol. Chem. 268: 11512-11515, 1993[Abstract/Free Full Text].
Benaksas, E. J., Murray, E. D., Jr., Rodgers, C. L., Pham, T., Bigornia, A. E., Dewind, S. A., Giebel, R., Brubacher, E. S. and Wechter, W. J.: Endogenous natriuretic factors 1: Sodium pump inhibition does not correlate with natriuretic or pressor activities from uremic urine. Life Sci. 52: 1045-1054, 1993[Medline].
Benaksas, E. J., Murray, E. D., Jr. and Wechter, W. J.: Natriuretic hormones II. Prog. Drug Res. 45: 245-288, 1995[Medline].
Burton, G. W. and Ingold, K. U.: Vitamin E as an in vitro and in vivo antioxidant. Ann. NY Acad. Sci. 570: 7-22, 1989[Medline].
Charlton, J. A. and Baylis, P. H.: Lack of inhibition of vasopressin-stimulated Na⁺K⁺ ATPase by atrial natriuretic factor in the rat renal medullary thick ascending limb of Henle's loop. Cell. Biochem. Funct. 8: 25-29, 1990[Medline].
Chiku, S., Hamamura, K. and Nakamura, T.: Novel urinary metabolite of d- $delta$ -tocopherol in rats. J. Lipid Res. 25: 40-48, 1984[Abstract].
Chiou, S. and Vesely, D. L.: Dimethyl sulfoxide inhibits renal Na⁺-K⁺-ATPase at a site different from ouabain and atrial peptides. Life Sci. 57: 945-955, 1995[Medline].
Crabos, M., Grichois, M. L., Guicheney, P., Wainer, I. W. and Cloix, J.: Further biochemical characterization of an Na⁺-pump inhibitor purified from human urine. Eur. J. Biochem. 162: 129-135, 1987[Medline].
de Wardener, H. E., Mills, I. H., Clapham, W. F. and Hayter, C. J.: Studies on the efferent mechanism of the sodium diuresis which follows the administration of intravenous saline in the dog. Clin. Sci. 21: 249-258, 1961[Medline].
Goto, A., Ishiguro, T., Yamada, K., Ishii, M., Yoshioka, M., Eugchi, C., Shimora, M. and Sugimoto, T.: Isolation of a urinary digitalis-like factor indistinguishable from digoxin. Biochem. Biophys. Res. Commun. 173: 1093-1101, 1990[Medline].
Greger, R. and Schlatter, E.: Presence of luminal K⁺, a prerequisite for active NaCl transport in the cortical thick ascending limb of Henle's loop of rabbit kidney. Pflugers Archiv. 392: 92-94, 1981[Medline].
Greger, R.: Ion transport mechanisms in thick ascending limb of Henle's loop of mammalian nephron. Physiol. Rev. 65: 760-797, 1985[Free Full Text].
Hebert, S. C. and Andreoli, T. E.: Control of NaCl transport in thick ascending limb. Am. J. Physiol. 246: F745-F756, 1984[Abstract/Free Full Text].
Kamal-Eldin, A. and Appelqvist, L.-Å.: The chemistry and antioxidant properties of tocopherols and tocotrienols. Lipids 31: 671-701, 1996[Medline].
Kantoci, D., Murray, E. D., Jr., DeWind, S. A., Borchardt, D., Khan, S. and Wechter, W. J.: Endogenous natriuretic factors 6: The stereochemistry of a natriuretic $gamma$ -tocopherol metabolite LLU- $alpha$ . J. Pharmacol. Exp. Ther. 282: 000-000, 1997.
Ludens, J. H., Clark, M. A., Ducharme, D. W., Harris, D. W., Lutzke, B. S., Mandel, F., Matthews, W. R., Sutler, D. M. and Hamlyn, J. M.: Purification of an endogenous digitalis-like factor from human plasma for structural analysis. Hypertension 17: 923-929, 1991[Abstract/Free Full Text].
Mathews, W. R., DuCharme, D. W., Hamlyn, J. M., Harris, D. W., Mandel, F., Clark, M. A. and Ludens, J. H.: Mass spectral characterization of an endogenous digitalislike factor from human plasma. Hypertension 17: 930-935, 1991[Abstract/Free Full Text].
Murray, E. D., Jr., Kantoci, D., DeWind, S. A., Bigornia, A. E., D'Amico, D. C., King, J. G., Jr., Pham, T., Levine, B. H., Jung, M. E. and Wechter, W. J.: Endogenous natriuretic factors 3: Isolation and characterization of human natriuretic factors LLU- $alpha$ , LLU- $beta$ ₁, and LLU- $gamma$ . Life Sci. 57: 2145-2161, 1995[Medline].
Pamnani, M. B., Chen, S., Bryant, H. J., Schooley, J. F., Jr., Eliades, D. C., Yuan, C. M. and Haddy, F. J.: Effects of three sodium-potassium adenosine triphosphatase inhibitors. Hypertension 18: 316-324, 1991[Abstract/Free Full Text].
Schönfeld, A., Schultz, M., Petrizka, M. and Gassman, B.: A novel metabolite of RRR- $alpha$ -tocopherol in human urine. Die Nahrung 37: 498-500, 1993[Medline].
Schultz, M., Leist, M., Petrzika, M., Gassmann, B. and Breigelius-Flohé, R.: Novel urinary metabolite of $alpha$ -tocopherol, 2,5,7,8-tetramethyl-2 (2 $'$ -carboxyethyl)-6-hydroxychroman, as an indicator of an adequate vitamin E supply? Am. J. Clin. Nutr. 62: suppl., 1527S-1534S, 1995.
Schwartzman, M. L. and McGiff, J. C.: Renal cytochrome P450. J. Lipid Med. Cell Sig. 12: 229-242, 1995[Medline].
Sekihara, H. and Yuzaki, Y.: Ouabain causes kaliuresis and works synergistically with aldosterone in vivo. Life Sci. 53: 975-980, 1993[Medline].
Simon, E. J., Gross, C. S. and Milhorat, A. T.: The metabolism of vitamin E. I. J. Biol. Chem. 221: 707-805, 1956a.
Simon, E. J., Eisengart, A., Sundheim, L. and Milhorat, A. T.: The metabolism of vitamin E. II. Purification and characterization of urinary metabolites of $alpha$ -tocopherol. J. Biol. Chem. 221: 807-817, 1956b[Free Full Text].
Smyth, D. D., Templeton, J. F., Sashi Kumar, V. P., Yan, Y., Widajewicz, W. and Labella, F. S.: Digitaloid pregnanes promote potassium-sparing diuresis in the guinea pig. Can. J. Physiol. Pharmacol. 70: 723-727, 1992[Medline].
Tymiak, A. A., Norman, J. A., Bolgar, M., DiDonato, G. C., Lee, H., Parker, W. L., Lo, L.-C., Berova, N., Nakanishi, K., Haber, E. and Haupert, G. T., Jr.: Physiochemical characterization of a ouabain isomer isolated from bovine hypothalamus. Proc. Natl. Acad. Sci. U.S.A. 90: 8189-8193, 1993[Abstract/Free Full Text].
Vereninov, A. A., Marakhova, I. I., Osipov, V. V. and Toropova, F. V.: Blast transformation of lymphocytes is accompanied by and increase in expression of mRNA, coding for Na, K-ATPase. FEBS Lett. 316: 37-40, 1993[Medline].
Wang, W. H.: Two types of K⁺ channel in thick ascending limb of rat kidney. Am. J. Physiol. 267: F599-F605, 1994[Abstract/Free Full Text].
Wang, W. H. and Lu, M.: Effect of arachidonic acid on activity of the apical K⁺ channel in the thick ascending limb of the rat kidney. J. Gen. Physiol. 106: 727-743, 1995[Abstract/Free Full Text].
Wechter, W. J. and Benaksas, E. J.: Natriuretic hormones. Prog. Drug Res. 34: 231-260, 1990[Medline].
Wechter, W. J., Kantoci, D., Murray, E. D., Jr., D'Amico, D. C., Jung, M. E. and Wang, W.-H.: A new endogenous natriuretic factor: LLU- $alpha$ . Proc. Natl. Acad. Sci. U.S.A. 93: 6002-6007, 1996a[Abstract/Free Full Text].
Wechter, W. J., Murray, E. D., Jr., Kantoci, D. and Jung, M. E.: Characterization of two new endogenous natriuretic factors. J. Am. Soc. Nephrol. 7: 1819, 1996b.
Zhao, N., Lo, L.-C., Berova, N., Nakanishi, K., Tymiak, A. A., Ludens, J. H. and Haupert, G. T., Jr.: Na, K-ATPase inhibitors from bovine hypothalamus and human plasma are different from ouabain: Nanogram scalde CD structural analysis. Biochemistry 34: 9893-9896, 1995[Medline].

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Endogenous Natriuretic Factors 7: Biospecificity of a Natriuretic -Tocopherol Metabolite LLU-1

Endogenous Natriuretic Factors 7: Biospecificity of a Natriuretic $gamma$ -Tocopherol Metabolite LLU- $alpha$ ¹