Oxytocin exerts harmful cardiac repolarization prolonging effects in drug-induced LQTS

Background Oxytocin is used therapeutically in psychiatric patients. Many of these also receive anti-depressant or anti-psychotic drugs causing acquired long-QT-syndrome (LQTS) by blocking HERG/IKr. We previously identified an oxytocin-induced QT-prolongation in LQT2 rabbits, indicating potential harmful effects of combined therapy. We thus aimed to analyze the effects of dual therapy with oxytocin and fluoxetine/risperidone on cardiac repolarization. Methods Effects of risperidone, fluoxetine and oxytocin on QT/QTc, short-term variability (STV) of QT, and APD were assessed in rabbits using in vivo ECG and ex vivo monophasic AP recordings in Langendorff-perfused hearts. Underlying mechanisms were assessed using patch clamp in isolated cardiomyocytes. Results Oxytocin, fluoxetine and risperidone prolonged QTc and APD in whole hearts. The combination of fluoxetine + oxytocin resulted in further QTc- and APD-prolongation, risperidone + oxytocin tended to increase QTc and APD compared to monotherapy. Temporal QT instability, STVQTc was increased by oxytocin, fluoxetine / fluoxetine + oxytocin and risperidone / risperidone + oxytocin. Similar APD-prolonging effects were confirmed in isolated cardiomyocytes due to differential effects of the compounds on repolarizing ion currents: Oxytocin reduced IKs, fluoxetine and risperidone reduced IKr, resulting in additive effects on IKtotal-tail. In addition, oxytocin reduced IK1, further reducing the repolarization reserve. Conclusion Oxytocin, risperidone and fluoxetine prolong QTc / APD. Combined treatment further prolongs QTc/APD due to differential effects on IKs and IK1 (block by oxytocin) and IKr (block by risperidone and fluoxetine), leading to pronounced impairment of repolarization reserve. Oxytocin should be used with caution in patients in the context of acquired LQTS.


Introduction
Congenital long QT syndrome (LQTS) -a rare genetic channelopathy with increased risk for lethal ventricular arrythmiasis caused by mutations in cardiac ion channels [1,2]. A similar, but more frequent form of QT prolongation, the acquired LQTS, is caused by a variety of drugs, which block repolarizing potassium currents, and shows similar clinical features (prolonged QTc and ventricular arrhythmias) as the inherited form [3]. I Kr current, conducted by HERG channels, is a key outward potassium current in phase-3-repolarization of the cardiac action potential and the main target for drugs causing acquired LQTS [4]. Antipsychotics, such as risperidone, as well as antidepressants, such as fluoxetine, block I Kr potentially leading to severe cardiac events such as torsade-de-pointes tachycardia or even sudden cardiac death [5,6].
Patients suffering from autism spectrum disorder and borderline personality disorder often receive drug treatment with risperidone or fluoxetine [7]. As an inherited impairment of the oxytocin system -that affects the brain with regard to cognitive and behavioral processes -is thought to be a key aspect regarding the etiology of these diseases [8], novel combined medical therapies with oxytocin are used in those patients. Oxytocin exerts anxiolytic effects, attenuates behavioural processes towards stress and promotes social functions such as trust, the socalled "bonding effect" [9,10]. Oxytocin, however, has also demonstrated QT-prolonging effects in human and animal studies [11][12][13][14]. We could previously demonstrate QT-prolonging and pro-arrhythmic effects in transgenic LQT2 rabbits [15].
In the current study, we aimed at elucidating potential QT-/APDprolongation and resulting pro-arrhythmia indicators by combined treatment with oxytocin and risperidone or fluoxetine in wild-type rabbits, their explanted hearts and single cardiac myocytes. The rabbit was chosen as model system due to pronounced species similarities in cardiac repolarizing ion currents between humans and rabbits [16] that facilitate future translation to human subjects.

Methods
A more detailed method description can be found in the online supplement.

Animal studies
All animal experiments were performed in accordance with the German animal protection law (TierSchG) and the Directive 2010/63/ EU of the European Parliament after approval by the local authorities (Regierungspräsidium Freiburg; protocol number G15/114). As female subjects and animals are more susceptible to drug-induced, acquired LQTS [17] only adult female wild type New Zealand White rabbits of similar age and weight were used for in vivo and ex vivo experiments.

Surface ECG
Surface ECG measurements were performed in sedated WT rabbits at baseline and with oxytocin (bolus 1.5 IU i.v., infusion with 1 IU/ml at a rate of 6 ml/h), with fluoxetine (bolus 1 mg/kg i.v., infusion with 2 mg/ ml at a rate of 4.5 ml/h) and risperidone (bolus 0.3 mg/kg i.v., infusion with 0.3 mg/ml at a rate of 10 ml/h). As we have previously demonstrated stable QTc values in temporal "sham" control measurements over > 30 min [15], no temporal control at baseline conditions were performed. I.v.-injection was used to ensure adequate blood concentration of the different compounds and to avoid uncertainties in serum concentrations following oral administration that may stem from species differences in pharmacokinetics.

Isolation of rabbit ventricular cardiomyocytes
Standard collagenase digestion was used to isolate ventricular cardiomyocytes [18]. After anesthesia and euthanasia as described above, rabbit hearts were rapidly excised, mounted on a Langendorff apparatus, and perfused with oxygenated, 37 • C warm Tyrode solution supplemented with 0.8-1 mg/mL collagenase (Worthington type 2) and 33 µM Ca 2+ for 25-40 min.

Electrophysiological recording in rabbit cardiomyocytes
To assess the effects of the compounds on AP and ion currents, patch clamp experiments were performed using Axopatch 200B patch clamp amplifier (Molecular Devices) and pCLAMP software (Axon Instruments).
APs were recorded in current clamp with 2-3 ms 0.4 mA square pulses at 0.5, 1 and 2 Hz. Membrane currents were recorded using the whole cell configuration. For studies of I K (I Kr + I Ks ), and I K1 cardiomyocytes were superfused with normal Tyrode solution. To measure I Kr , I Ca,L and I Ks were inhibited by 1 µM nisoldipine (Sigma) and 30 µM chromanol 293B (Sigma). I-V relationship for I K and I Kr tail currents were determined by applying 1.5 s depolarizing voltage pulses from holding potential of − 40 mV to test potentials ranging from − 30 to + 60 mV. Tail current was measured upon repolarization to − 40 mV. I K1 was elicited from a holding potential of − 20 mV by voltage steps from − 120 mV to + 50 mV. Steady-state I K1 amplitudes were estimated at the end of the 500 ms pulse. All experiments were carried out at room temperature.

Surface ECG
To assess in vivo effects of oxytocin and its combination with psychopharmaceutic drugs on QT intervals, surface ECG were measured.

Changes in QT and RR over time
Oxytocin (n = 13), fluoxetine (n = 23), risperidone (n = 21) and their combination with oxytocin all prolonged QT duration compared to baseline (Suppl. Fig. 1A-C) -with a more pronounced QT prolongation upon combined exposure. As heart rate slowed during the experiments (particularly during oxytocin (Suppl. Fig. 1A-C) but also during fluoxetine perfusion (Suppl. Fig. 1B)), heart-rate corrected QT durations were calculated (QTc).

QTc duration
Application of oxytocin resulted in a significant increase of mean QTc duration compared to baseline in WT ( Fig. 1A; comparison at 20 min after exposure). Similarly, fluoxetine (Fig. 1B), risperidone (Fig. 1C) or their combination with oxytocin significantly prolonged QTc. Important to note, a significant difference between the QT-prolonging effect of fluoxetine alone and fluoxetine + oxytocin (fluo + oxy) and between risperidone alone and risperidone + oxytocin (risp + oxy) was observed ( Fig. 1) with a further prolongation in the combined treatment. On the right-hand side of Fig. 1A-C the individual prolongation of QTc duration compared to baseline is shown for each individual rabbit, indicating that this prolongation is seen among all animals.

Short term variability (STV)
To elucidate potential pro-arrhythmic effects of the individual compounds, short term variability of QTc -a marker for temporal heterogeneity of repolarization -was assessed [19]. Oxytocin alone, fluoxetine and risperidone as well as their combination with oxytocin significantly increased STV QTc compared to baseline ( Fig. 2A-B), indicating a pro-arrhythmic potential. While the combined treatment with antipsychotic/depressant drugs and oxytocin also induced an increased STV QTc compared to baseline, no differences could be observed between fluoxetine and risperidone and their combinations with oxytocin ( Fig. 2A-B).

Monophasic action potential recordings
Monophasic action potentials in isolated Langendorff-perfused rabbit hearts were used to determine ex vivo effects on cardiac repolarization in whole hearts.

Monophasic action potential duration
Mean APD 75 measured at 2 Hz stimulation frequency was significantly prolonged in oxytocin-perfused hearts compared to baseline (Fig. 3A).
Fluoxetine and fluoxetine + oxytocin also prolonged mean APD 75 compared to baseline (Fig. 2B). Importantly, the combined treatment with oxytocin and fluoxetine significantly prolonged mean APD 75 compared to fluoxetine alone (Fig. 3B) -but did not lead to a potentiation of the APD-prolongation.
Similarly, risperidone and risperidone + oxytocin increased mean APD 75 compared to baseline (Fig. 3C). However only a trend towards a further prolongation could be observed by the combination of risperidone + oxytocin compared to risperidone alone.
Fluoxetine (3 µM) also prolonged APD compared to baseline (Fig. 3E). In a subset of cells, in which a combination of fluoxetine + oxytocin was applied, fluoxetine + oxytocin slightly (but nonsignificantly) prolonged APD compared to baseline and the APD prolonging effect of combination of fluoxetine + oxytocin tended to be more pronounced than fluoxetine alone (p = 0.07, Fig. 3E).
Similarly, risperidone (1 µM) prolonged APD compared to baseline (Fig. 3F). In a subset of cells, in which a combination of risperidone + oxytocin was applied, risperidone + oxytocin also tended to prolong APD compared to baseline and, importantly, the risperidone + oxytocin combination significantly prolonged APD compared to risperidone alone (Fig. 3F).
None of the hormones/drugs affected resting membrane potential (RMP), action potential amplitude (APA) and the maximum velocity of depolarization (dV/dt max , V max )

Underlying mechanisms -effects on repolarizing ion currents
To reveal the underlying ionic mechanisms of the prolongation in APD after risperidone, fluoxetine and their combination with oxytocin, we focused on studying the (total) delayed rectifier current (I K -a composite of I Ks and I Kr ) since previous studies have indicated that risperidone and fluoxetine block I Kr [5,6], while we have demonstrated that oxytocin does not affect I Kr , but causes a significant decrease in I Ks [15) (Fig. 4).
In Fig. 4, these effects of oxytocin are summarized: oxytocin did not alter I Kr -tail currents (Fig. 4B). In contrast, oxytocin significantly reduced I Ks -tail by approximately 47% at + 40 mV (Fig. 4A). The decrease in I Ks -steady (end-pulse) was less pronounced, approximately -33% at + 40 mV. The electrophysiological effects of fluoxetine and risperidone in cardiomyocytes had been previously studied extensively -demonstrating direct I Kr -blocking properties in cardiomyocytes of various species and resulting APD-and QT-prolonging effects [20][21][22][23][24]. We therefore conducted measurements of fluoxetine and risperidone effects on I Kr only in limited number of cells, in which we confirmed previous results regarding I Kr -blockade (Suppl. Fig. 2): Fluoxetine (3 µM) decreased I Kr-tail at + 40 mV by 47%. Risperidone (1 µM) decreased I Kr-tail at + 40 mV by 28%.
Oxytocin decreased I Ktotal -tail at + 40 mV by 34% (Fig. 5). Fluoxetine decreased I Ktotal -tail at + 40 mV by 67% (Fig. 5). When a combination of fluoxetine + oxytocin was applied, the inhibition was slightly bigger than fluoxetine alone (70% in I K -tail at + 40 mV Fig. 3). Risperidone alone blocked I K -tail at + 40 mV by 55.5% (Fig. 5). When a combination of risperidone + oxytocin was applied, the inhibition of I K -tail at + 40 mV was more pronounced than with risperidone alone (74%, Fig. 5), indicating the oxytocin-induced I Ks block and the fluoxetine + risperidone induced I Kr block are additive on repolarizing total I K .
The differential I Ks /I Kr -blocking effects of the compounds were also apparent when comparing their APD-prolonging effects at different frequencies. The I Ks blocker oxytocin, exerted an APD-prolongation without frequency-dependence with similar APD prolongation at 0.5, 1, and 2 Hz (Suppl. Fig. 3A). Risperidone on the other hand behaved like a classical I Kr -blocker with reverse frequency-dependence [22] and caused a clear APD-prolongation at 1 Hz and no significant APD prolongation at 2 Hz (Suppl. Fig. 3B). Despite being also an I Kr -blocker (but also with other ion channel blocking properties) fluoxetine had no reverse frequency-dependence with similar APD-prolongation at 0.5 Hz and 1 Hz (Suppl. Fig. 3C) -as previously described [24,25].
In addition, we investigated the potential electrophysiological effects on the inward rectifier potassium current (I K1 ) (Fig. 6). Oxytocin reduced I K1 at negative membrane potentials (from − 120 to − 90 mV, Fig. 6), thus further reducing the repolarization reserve in cardiomyocytes, while risperidone and fluoxetine alone had no effects on I K1 (Fig. 6). The combination of oxytocin with risperidone or with fluoxetine showed similar I K1 blocking effects as oxytocin alone (Fig. 6).

Discussion
Drug-induced LQTS remains an important and feared pharmacological side effect of a variety of drugs. This study demonstrated potentially harmful repolarization prolonging effects of the "binding-hormone" oxytocin, the anti-depressant fluoxetine, the anti-psychotic risperidone, and -particularly -their combination that is clinically used in various psychiatric disorders and elucidated the underlying mechanisms.

QT interval and other in vivo pro-arrhythmia markers
The evaluation of in vivo pro-arrhythmia markers such as QTc plays a

Fig. 2. Drug and hormone effects on short-term variability of QTc (STV QTc ). A.
Examples of Pointcaré plots indicating STV QTc at baseline, and during administration of oxytocin, fluoxetine, fluoxetine + oxytocin, risperidone, and risperidone + oxytocin. B. Dot plots indicating changes in STV QTc following application of oxytocin (n = 9), fluoxetine and fluoxetine + oxytocin (n = 9), risperidone and risperidone + oxytocin (n = 10). Differences are indicated as * p < 0.05; ** p < 0.01; ***p < 0.001. major role in risk stratification for congenital and drug-induced LQTS [3,26]. The combination of two or more QT-prolonging drugs is a known risk factor for drug-induced LQTS and resulting drug-induced proarrhythmia [27,28]. However, this has mostly been demonstrated for the combination of several drugs blocking I Kr .

Fig. 3. Drug and hormone effects on APD in perfused hearts and isolated cardiomyocytes. A-C. Effects on monophasic APD acquired in
In this study, we demonstrated significant QTc prolonging effects of risperidone and fluoxetine as single drugs in wildtype rabbits, which is consistent with previous findings and case reports in human subjects [5,23] -particularly following risperidone, while the QT-prolonging effects of fluoxetine seem to be more variable in individual patients [29,30]. Likewise, oxytocin monotherapy significantly prolonged QTc in wildtype rabbits, similarly as in previous case reports and animal studies that have shown QTc-prolongation both in normal subjects and -more pronouncedly -in the setting of reduced repolarization reserve as in LQTS or in chronic-ischemia induced APD-prolongation [11,31]. Along these lines, we recently demonstrated that oxytocin also prolongs QT and cellular APD in transgenic LQT2 rabbits and identified I Ks blocking properties of oxytocin as the underlying electrophysiological mechanism [15].
We here demonstrated an additive effect of I Ks blocking oxytocin and the anti-depressant fluoxetine or the anti-psychotic risperidone on QTc, causing more pronounced prolongation upon combined treatment compared to monotherapy. The term "repolarization reserve" indicates the ability of cardiomyocytes to maintain sufficient repolarization despite repolarization-prolonging effects by compounds due to a compensation via non-affected "reserve" K + currents [32]. Risperidone and fluoxetine block I Kr [5,6]. The additional blockade of I Ks through oxytocin thus leads to a further reduction of this repolarization reserve. This combination of a blockade of different ion currents can explain the enhanced prolongation of repolarization seen in this study.
While the question concerning an increased pro-arrhythmic effect of fluoxetine or risperidone monotherapy remains unanswered with contradictory evidence [3,33] the combination with another QT-prolonging compound, such as oxytocin, could severely increase the risk for arrhythmia, especially by affecting different ion channels rather than the same. With the concept of the repolarization reserve in mind, a combination of risperidone or fluoxetine plus oxytocin reduces the repolarization reserve in such manner that arrhythmia development becomes more likely [27]. Important to note, however, only additive effects and no potentiation were seen during combined treatment, which may indicate a less pronounced pro-arrhythmic potential than in case of combined treatment with pure I Kr -and I Ks -blockers as in the classical experiments conducted by Biliczki et al. with dofetilide and chromanol [34].
In addition to QTc, we have investigated other markers of proarrhythmia: Beat-to-beat short-term variability of QTc (STVQT), which indicates temporal instability in cardiac repolarization and is a novel marker regarding risk stratification of cardiac arrhythmias. Increased STVQT is associated with higher risk for arrhythmia and could be used as a predictive marker [19]. In animal studies, alteration of STVQT was assessed both for I Kr and I Ks blockers, showing similar results in the extent of increase of STVQT [35,36]. Especially the combination of both, I Kr and I Ks blockade, showed significantly increased and clinically relevant beat-to-beat variability [36]. Oxytocin, risperidone and fluoxetine significantly increased STV QTc , therefore underlining the proarrhythmic properties of these compounds and their combination.
Though we did not observe any spontaneous arrhythmias or early afterdepolarizations directly, we could previously demonstrate reduced repolarization reserve and increased propensity to pro-arrhythmic permanent depolarization, lack of 1:1 capture and early afterdepolarization formation in an in silico computational LQT2 model with lack of I Kr , in which we have incorporated the experimentally observed acute oxytocin effects [15]. Therefore, one may assume that in the context of acquired LQTS due to I Kr -blocking drugs (such as fluoxetine or risperidone) in combination with oxytocin, similar pro-arrhythmic events may occur.

Monophasic action potential duration in Langendorff-perfused hearts
Drug-induced prolongation of APD is considered a risk factor for the development of pro-arrhythmic early afterdepolarizations (EADs) and resulting arrhythmias [37]. On the whole heart level, risperidone / fluoxetine, and oxytocin prolonged monophasic APD -in line with the in vivo QT effects observed in our study. This observation is similar to previous studies [15,33]. Moreover, we demonstrated that the combined treatment with oxytocin and fluoxetine significantly prolonged monophasic APD compared to fluoxetine alone and that for the combined treatment of risperidone and oxytocin a similar trend was observed, thus indicating additive effects of the combined treatment on cardiac repolarization -similarly as observed in vivo.

Underlying electrophysiological mechanisms
As demonstrated in heterologous HERG-expression systems and cardiomyocytes, risperidone is a potent blocker of I Kr [5,22,23] and has a potent lengthening effect on cardiac repolarization (QT, APD) at clinically relevant drug concentrations [23]. Similarly, we confirmed I Kr -blocking effects of risperidone in rabbit cardiomyocytes and pronounced reduction of I Kr and I K total, which explain the observed QTand APD-prolonging effects.
Similarly, fluoxetine -a multichannel blocker -also blocks I Kr at clinically relevant concentrations [6] and thereby prolongs APD/QT. The repolarization prolonging effects are, however, not as pronounced as fluoxetine also inhibits the L-type calcium channel (I Ca,L ) [24]. In our rabbit models, however, fluoxetine consistently prolonged QT and monophasic APD due to its effects on I Kr and I Ktotal .
Oxytocin exerts its QT and APD prolonging effects via a different mechanism. As we have previously demonstrated, oxytocin does not affect I Kr but reduces I Ks -steady and I Ks -tail currents [15]. Additionally, we could demonstrate here that oxytocin may also reduce I K1 at very negative membrane potentials (-90 to − 120 mV), thereby further decreasing the repolarization reserve. The oxytocin-induced reduction of I K1 at very negative potentials willtheoreticallynot directly prolong the QT/APD. The decrease of the inward component of I K1 , however, may influence both active and passive membrane properties. Additionally, it could increase the resting membrane resistance together with membrane hypopolarization. Consequently, this could finally increase the likelihood of reaching threshold potentials, thus increasing the probability of AP discharge.
The additive effect of oxytocin and the anti-depressant fluoxetine or the anti-psychotic risperidone on cardiac repolarization (QT/APD) with more pronounced prolongation upon combined treatment compared to monotherapy can be explained by the different mechanisms via which the different drugs / hormones exert their effects on cardiac repolarization: risperidone and fluoxetine mainly block I Kr [5,6], and the additional blockade of I Ks through oxytocin leads to a further reduction of the "repolarization reserve". Important to note, the effect of both risperidone and fluoxetine on cellular APD was less pronounced than the effects observed in the Langendorff-perfused hearts. This might be partially due to differences in the temperature at which cellular AP and MAP were acquired, as ion current characteristics are known to be affected by changes in temperature. Additionally, isolated cells are not coupled, while cardiomyocytes within the tissue are coupled to each other. The latter (more physiological situation) may change AP morphology due to the electrotonic sink, which again will indirectly change the relative contribution of individual ion currents [38] and thereby the effects of drugs on APD.
Indeed, similarly as in our cellular experiments, other studies observed very heterogenous effects on cellular APD ranging from clear APD prolongation to nearly no APD prolongation (or even sometimes APD-shortening by fluoxetine) in some preparations [5,22,24,39,40] despite consistent I Kr -block -likely due to the additional I Ca.L blocking effects of both drugs -which will lead to a shortening of APD and will counteract the block of risperidone and fluoxetine on I Kr , which otherwise would lead to a prolongation of APD in rabbit cardiomyocytes. Indeed, despite the pronounced inhibition of I K by risperidone and fluoxetine that was observed in all rabbit cardiomyocytes investigated, in our experimental settingsimilarly as in previous reports -in roughly 25% of isolated rabbit cardiomyocytes APD 50 and APD 90 was not prolonged after risperidone or fluoxetine treatment. This resulted in slight discrepancies between the extent of cardiac repolarization-prolonging effects between drug-induced QTc prolongation and cellular APD prolongation. For example, risperidone and risperidone + oxytocin prolonged QTc by 13% and 19%; while in patch clamp experiments, risperidone + oxytocin only prolonged cellular APD 90 by 5%. Interestingly, in case of fluoxetine the QTc changes were comparable with APD 90 data obtained in patch clamp experiments. Importantly, a similar %-prolongation of QTc (and APD) by risperidone and fluoxetine was also observed in other species such as cats and dogs [20,22].
These data indicate that it is very important to also assess the effects of drugs or drug-combinations not only on cellular level, but also in the whole heart and the intact animal to fully investigate their potential proarrhythmic cardiac repolarization.
It is not yet known how oxytocin blocks KCNQ1/I Ks on the molecular level. Theoretically, the effects could be exerted by direct blockade through an interaction with the channel protein or by an alteration of the KCNQ1/I Ks expression via oxytocin-receptors. As the first I Ks decreasing effects are seen within a very short time (~2min) of oxytocin perfusion, a direct interaction seems to be plausible. Thus far, however, it is not known in which region of the channel protein this interaction may occur. In addition, we could previously demonstrate that changes in the expression of various channel occur in case of more chronic exposure -such as an increase in mRNA and protein levels of CACNA1C/Ca v 1.2 and RyR2 -which may further aggravate acute effects on cardiac repolarization.

Clinical implications
Patients receiving more than one QT-prolonging drug bear an increased risk for cardiac arrhythmias. Administration of multidrugtreatment should be considered carefully especially in the context of drug-induced acquired LQTS. As this study suggests an additive effect on QT-prolongation when the "bonding-hormone" oxytocin -which has emerged as promising drug for a variety of psychiatric disorders -is combined with risperidone or fluoxetine, the indication for such a combined treatment should be considered carefully, and ECG / QT duration should be monitored regularly during treatment (particularly in situations in which additional pro-arrhythmic factors are present such as electrolyte imbalances). Important to note, however, only additive effects and no potentiation were seen during combined treatment, which may indicate a less pronounced pro-arrhythmic potential than in case of combined treatment with pure I Kr -and I Ks -blockers [34].

Limitations
Only adult female rabbits were used for the experiments, as both women and female rabbits are known to be more sensitive to I Kr -blocker induced drug-induced QT-prolongation than males [3]. Some studies indicate that QT-prolonging effects of oxytocin might be more pronounced in male rabbits [11]; hence the effect of oxytocin and combined treatment found in this study might differ between sexes.
Although rabbits show pronounced similarities with humans in cardiac electrophysiology [16] some species differences always exist, indicating that confirmatory studies in human subjects are warranted to evaluate the exact effect of combined treatment with oxytocin and psychiatric medication in human subjects. Additionally, the parameters investigated in this study are only indirect parameters for proarrhythmic properties of the drug combinations. Larger scale studies investigating the pro-arrhythmic effects of oxytocin, fluoxetine, risperidone and their combination with oxytocin directly need to be performed to further elucidate the clinical pro-arrhythmic potential of these drug combinations.

Conclusion
Treatment with multiple repolarization prolonging drugs is a main risk factor for patients to develop drug-induced acquired LQTS with potential malignant outcome. This study provides evidence that the hormone oxytocin prolongs QTc / APD and increases temporal heterogeneity of repolarization caused by I Ks blockade. Combined treatment of the I Ks -blocking drug oxytocin with the antipsychotic I Kr -blocking drug risperidone or the antidepressant I Kr -blocking drug fluoxetine showed additional increase in QTc interval and APD, suggesting a potential harmful interaction in combined drug use.