5-aminolevulinic acid (ALA) is utilized in a photodynamic therapy as a compound capable of augmenting intracellular pool of protoporphyrin IX (PpIX), which exhibits properties of a photosensitizer. The studies were aimed at monitoring accumulation of endogenous protoporphyrin IX in CHO cells under effect of various concentrations of ALA in culture medium and following removal of the compound from the culture medium. Cell content of PpIX was determined following incubation of the cells for 72 h in a culture medium containing different concentration of ALA. Moreover, the cells were preincubated for 2 h in ALA at various concentrations and separated from the compound by medium change and their PpIX content was monitored following incubation. PpIX content was defined by a fluorescent technique under the confocal microscope. In the course of continuous incubation of cells with ALA, biphasic alterations were noted in cellular PpIX concentration. Removal of ALA from the incubation medium resulted at first in a decrease in PpIX content in cells, which was followed by an evidently augmented accumulation of the compound in the cells. The results suggested that in the case of CHO cells, exogenous ALA was not an exclusive source of PpIX synthesis and that alterations in enzyme activities were responsible for production of PpIX

Warchoł, W

Wołuń-Cholewa, M

English

Via Medica Journals

FOLIA HISTOCHEMICAET CYTOBIOLOGICAVol. 42, No. 2, 2004pp. 131-135Effect of 5-aminolevulinic acid on kinetics of protoporphyrin IX production in CHO cellsM. Wołun´-Cholewa1 and W. Warchoł21Department of Radiobiology and Cell Biology and 2Department of Biophysics, University of Medical Sciences, Poznan´, PolandAbstract: 5-aminolevulinic acid (ALA) is utilized in a photodynamic therapy as a compound capable of augmentingintracellular pool of protoporphyrin IX (PpIX), which exhibits properties of a photosensitizer. The studies were aimed atmonitoring accumulation of endogenous protoporphyrin IX in CHO cells under effect of various concentrations of ALA inculture medium and following removal of the compound from the culture medium. Cell content of PpIX was determinedfollowing incubation of the cells for 72 h in a culture medium containing different concentration of ALA. Moreover, the cellswere preincubated for 2 h in ALA at various concentrations and separated from the compound by medium change and theirPpIX content was monitored following incubation. PpIX content was defined by a fluorescent technique under the confocalmicroscope. In the course of continuous incubation of cells with ALA, biphasic alterations were noted in cellular PpIXconcentration. Removal of ALA from the incubation medium resulted at first in a decrease in PpIX content in cells, which wasfollowed by an evidently augmented accumulation of the compound in the cells. The results suggested that in the case of CHOcells, exogenous ALA was not an exclusive source of PpIX synthesis and that alterations in enzyme activities were responsiblefor production of PpIX. Key words: Protoporphyrin IX - 5-aminolevulinic acid - CHO cells - Photodynamic therapyIntroductionPhotodynamic therapy (PDT) represents a therapeutictechnique, in which cytotoxic effects in cells are inducedby light. It requires that the cells contain a photosen-sitiser which induces the photochemical reactions lead-ing to destruction of the cells [15]. Photosensitizers canbe introduced to the cells exogenously, or from an en-dogenous source [12]. In the latter situation, protopor-phyrin IX (PpIX) is used, which accumulates in cellsunder the effect of 5-aminolevulinic acid (ALA), par-ticularly in neoplastic cells [2, 4, 7, 8]. ALA is a physi-ological precursor in the synthesis of heme, which is theporphyrin molecule (PpIX) with an iron atom in itsferrous state incorporated into its core. Free heme nega-tively regulates the activity of the enzyme ALA-syn-thase, which catalyses the initial metabolic step [1].Addition of exogenous ALA circumvents this negativefeedback control and induces an immediate increase inheme synthesizing activity, which results in intracellularaccumulation of PpIX. Photodynamic therapy based onALA application is at present increasingly widely ap-plied in clinical practice [5]. Till now, particular attention has been paid to theway, in which PpIX is distributed and accumulated incells under the effect of ALA, which undoubtedly hasformed the basis for defining mechanisms linked to PDTeffects [6, 10, 12]. For induction of a clinical effect it isimportant to recognise the kinetics of PpIX accumula-tion in cells, as influenced by the applied dose of ALA.Cellular content of the photosensitizer should be optimalfor induction of the photodestructive effect, followinglight exposure of the treated neoplastic lesions. Thekinetics of PpIX formation under the effect of exogenousALA is thought to result from circumvented bottle-necklinked to synthesis of endogenous ALA, the level ofwhich remains under control of free heme [1, 8, 11]. Considering that these problems may not only be oftheoretical significance, but also have a practical valuefor establishing conditions of a photodynamic therapy,we decided to define kinetics of PpIX accumulation inCHO cells under the effect of various concentrations ofALA. Moreover, we decided to examine if applicationof extracellular ALA affects endogenous mechanisms ofPpIX formation.Correspondence: M. Wołun´-Cholewa, Dept. Radiobiology andCell Biology, University of Medical Sciences, S´wie˛cickiego 6, 60-781 Poznan´, Poland; e-mail: doskon@amp.edu.plMaterials and methodsThe studies were performed on tumour CHO (Chinese HamsterOvary) cells, grown in RPMI 1640 supplemented with 100 g/mlstreptomycin, 100 U/ml penicillin, 2 mmol/l L-glutamine and 5%FCS in a controlled CO2 atmosphere (5%), at 37˚C. Effects of5-aminolevulinic acid (ALA) concentration on accumulation ofprotoporphyrin IX in CHO cells were defined by continuous incuba-tion of the cells in ALA concentrations of 1, 2.5 or 5 mmol/l culturemedium for the period of 0, 1, 2, 4, 8, 18, 24, 48 or 72 h. Followingthat time, PpIX content in cells was evaluated using a confocalmicroscope (LSM 510, Zeiss). The estimations took advantage ofPpIX-exciting laser beam of 458 nm wavelength (argon laser, HFT458), while the emitted light was analysed using 585 nm filter (LP585). Patterns of the analysed cells were captured using 512 × 512 pixelmeasuring window (0.0530 mm2) and the immersion fluorescenceobjective Plan-Neofluar 40×/1.3 Oil. Alterations in cellular PpIXcontent after removal of ALA from the incubation medium weredefined in the following manner: CHO cells subjected to 2 h prein-cubation with ALA (the time was selected in a preceding experiment)at concentrations of 1, 2.5 or 5 mmol/l culture medium were washedthrice and placed in the same medium for another 0, 2, 4, 8, 18, 24,48 or 72 h. After that time, PpIX content in cells was estimated byconfocal microscopy in the above described procedure. In eachexperiment, cells of control group, incubated in the same way, but inthe culture medium devoid of ALA were evaluated. PpIX content was evaluated using the CytFlu 1.2 software andexpressed in equipment units (e.u.), which reflected an averageintensity of fluorescence per cross-section area of the analysed cells(1 mm2). Each experiment was performed in 10 independent cul-tures. Statistical evaluation of the obtained results included theKruskal-Wallis test (nonparametric ANOVA), performed using Stat-istica ver. 5 software. P value <0.05 was considered significant.ResultsAt all tested ALA concentrations, continuous incubationof CHO cells resulted in a significant intensity increaseof PpIX fluorescence. Results of PpIX-specific fluores-cence estimation in a confocal microscope followingcontinuous incubation with ALA are presented in Figure1. At any of the applied ALA concentration, the relationbetween fluorescence in the examined cells and durationof incubation showed a biphasic character. Following 2h incubation, augmented values of fluorescence wereobserved in cells: to 1262 e.u. for ALA concentration of1 mmol/l, to 1350 e.u. for ALA concentration of 2.5mmol/l and to 1504 e.u. for ALA concentration of 5mmol/l. Intensities of the fluorescence differed onlyslightly between individual groups, despite clear dif-ferences in the applied ALA concentrations. In the sub-sequent 8 h of the experiment, intensity of thePpIX-specific fluorescence significantly decreased(p<0.001) and, then, slightly significantly increased(p<0.05) (particularly in cases of ALA concentrations of1 and 2.5 mmol/l) to significantly decrease again(p<0.05). At ALA concentration of 5 mmol/l, the peakfluorescence (1956 e.u.) was noted in 48th h of theexperiment (Fig. 2). PpIX-specific fluorescence in cellsof the control group did not significantly change in thecourse of the entire experiment and never exceeded thevalue of 85 e.u. A separate cycle of experiments was devoted toalterations in PpIX content in CHO cells, which werepreincubated with ALA for 2 h and then transferred tothe medium free of ALA. The obtained results are illus-trated in Figure 2. Following incubation with 1 mmol/lALA, the content of PpIX significantly decreased (from1262 to 548 e.u., p<0.01) 2 h after removal of ALA. Anaugmented content of PpIX was observed after 18 h(p<0.001), with gradual significant decrease (p<0.05) inthe subsequent hours of the experiment (Fig. 2). Like-wise, in the case of 2.5 mmol/l ALA a significant de-crease (p<0.05) in cellular PpIX content was noted 2 hfollowing transfer of the cells to ALA-free medium.However, subsequent hours brought about a significantincrease (p<0.001) in cellular PpIX content until 18 h ofincubation, when the content reached 3547 e.u. This wasfollowed by a logarithmic significant decrease(p<0.001) in cellular PpIX content. Two-hour incuba-tion of the cells with 5 mmol/l ALA was followed by,on the average, a threefold significant decrease (p<0.05)in cellular PpIX content 2 h following transfer of thecells to the ALA-free medium. In the subsequent timeperiod, cellular content of the compound gradually in-creased and between hours 8 and 24 of the incubation itpersisted at the levels of 1082 to 1589 e.u. (Fig. 2).DiscussionProperly conducted PDT initially requires an appropri-ate concentration of a photosensitizer and time whichhas to elapse between its application and light exposure.Accordingly, several studies have been focused on ac-cumulation of photosensitizers in cells depending upontheir physicochemical properties and their capacity topenetrate into the cells [4, 14]. The finding, that 5-ami-nolevulinic acid (ALA), which basically is not aphotosensitizer itself, induces accumulation in cells(particularly tumour cells) of endogenous protopor-phyrin IX has proved especially significant. Accumula-tion of PpIX in cells under the effect of ALA used to beevaluated by analysis of fluorescence intensity, em-ploying either culture material or cryostat sections,which as a rule, was hampered by a significant measure-ment error. In our studies, the measurements of fluores-cence intensity were performed using a confocalmicroscope, therefore the results reflect a thickness ofthe optical layer and not the total thickness of the exam-ined material in optical axis of the microscope. This hasallowed to obtain more reproducible results. The results have demonstrated that incubation inmedia containing 1, 2.5 or 5 mmol/l ALA did not induceaccumulation of PpIX in the cells, which would parallelthe applied ALA concentrations. Moreover, applicationof extreme, five-fold higher ALA concentrations re-132 M. Wołun´-Cholewa, W. Warchołsulted in an increase in PpIX-related fluorescence onlyby 6-10%. Similar results were noted in in vitro studieson human cell lines, originating from lung and bladdercancers, in which application of higher than optimal ALAconcentration resulted in a decrease in PpIX formation,paralleled by a decreased activity of mitochondria andlowered cell viability [14]. Continuous incubation of cellswith ALA brought about biphasic changes in PpIX meanfluorescence related to duration of the incubation. Theevident increase in the fluorescence intensity following2 h incubation was followed by its decrease (after 8 h),increase and another decrease. The observed alterationsshould be interpreted as a result of equilibrium betweensynthesis of PpIX in the cells and removal of PpIX dueto the binding of the compound to iron, its transforma-tion to heme or its efflux out of the cells [2]. Fig. 1. Alterations in PpIX content inCHO cells during continuous incuba-tion with ALA.Protoporphyrin IX production in CHO cells 133The rate of PpIX formation is controlled by theslowest reactions of the biosynthetic pathway and mayvary in different cells. At the preliminary stage of PpIXbiosynthesis, 5-aminolevulinic acid is synthesized in themitochondrial matrix from glycine and succinylCoAunder the effect of ALA-synthase. Subsequently, ALAfinds its way to the cytoplasm, in which in the presenceof ALA-dehydratase (ALA-D) it becomes condensed toporphobilinogen. As the result of subsequent reactions(deamination, decarboxylation and oxidation), catalysedby appropriate enzymes (porphobilinogen deaminase,uroporphyrinogen decarboxylase, coproporphyrinogenoxidase and protoporphyrinogen oxidase) PpIX isformed, from which, following addition of iron (ferro-chelatase - mitochondria), heme is produced [10]. Incases of augmented heme production, activity of ALA-Fig. 2. Alterations in PpIX content inCHO cells, which were preincubatedwith ALA for 2 h and then trans-ferred to the medium free of ALA.134 M. Wołun´-Cholewa, W. Warchołsynthase is inhibited due to a negative feedback [3]. Forthat reason, the cells do not accumulate intermediateproducts of PpIX synthesis or heme. Considering the above biosynthetic pathway of PpIXand heme, the ALA incubation-related augmented syn-thesis of PpIX in the cells could be interpreted as aneffect of bypassing the exogenous ALA of the slowestreaction which controls the dynamics of PpIX formation[7]. In such a situation, one should expect that increasedcontent of PpIX should develop as a second-order reac-tion and the maximum value should for certain timeexhibit plateau, as long as the synthesis of PpIX willbalance off its elimination. In cases of several cell lines,the change in PpIX content with duration of incubationwith ALA corresponded in fact to the kinetics of second-order reactions, thus indicating that ALA evidently par-ticipated in PpIX synthesis [9, 13]. In contrast, in ourstudies changes in PpIX concentration in the first 8 hoursof the experiment have corresponded to alterations,which used to be noted in sequential reactions, in whicha product of one reaction serves as a substrate for thesubsequent reaction. Similar results could be noted instudies of other authors [14]. The decrease in PpIXcontent in the studied CHO cells might have reflectedefflux of the compound or increased activity of ferroche-latase, which catalyses binding of PpIX with iron. In order to examine if exogenous ALA has beenresponsible for the observed effects, we performed theexperiments, in which ALA was removed from themedium following 2 h exposure of the cells and sub-sequent alterations in PpIX content were recorded. Ascompared to continuous exposure of cells to the com-pound, removal of ALA from the medium was followedby evident decrease in the photosensitizer-specific fluo-rescence in the cells. This has confirmed our expectationthat the augmented PpIX concentration in the first hoursof the experiment has reflected action of exogenousALA. Surprisingly, at later times following removal ofALA from incubation medium, augmented content ofPpIX was detected; even higher levels were observedthan in the medium containing ALA. At the moment, the mechanism of this phenomenonremains difficult to be interpreted, but one should keepin mind the potential for induction of enzymes respon-sible for ALA synthesis and possibly lower efflux of thecompound from the cells. It is certainly important forfuture investigations; it seems that in certain conditionsthe cell may preferentially switch to an endogenousmechanism, inducing a higher intracellular accumula-tion of the sensitizer.References[ 1] Batlle AMC (1993) Porphyrins, porphyrias, cancer and photo-dynamic therapy - a model for carcinogenesis. PhotochemPhotobiol 20: 5-22[ 2] Bartosova J, Hrkal Z (2000) Accumulation of protoporphyrin-IX (PpIX) in leukemic cell lines following induction by 5-ami-nolevulinic acid (ALA). 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Effect of 5-aminolevulinic acid on kinetics of protoporphyrin IX production in CHO cells.

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Effect of 5-aminolevulinic acid on kinetics of protoporphyrin IX production in CHO cells.

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