Unveiling the crucial role of betaine: modulation of GABA homeostasis via SLC6A1 transporter (GAT1)

Betaine is an endogenous osmolyte that exhibits therapeutic potential by mitigating various neurological disorders. However, the underlying cellular and molecular mechanisms responsible for its neuroprotective effects remain puzzling.In this study, we describe a possible mechanism behind the positive impact of betaine in preserving neurons from excitotoxicity. Here we demonstrate that betaine at low concentration modulates the GABA uptake by GAT1 (slc6a1), the predominant GABA transporter in the central nervous system. This modulation occurs through the temporal inhibition of the transporter, wherein prolonged occupancy by betaine impedes the swift transition of the transporter to the inward conformation. Importantly, the modulatory effect of betaine on GAT1 is reversible, as the blocking of GAT1 disappears with increased extracellular GABA. Using electrophysiology, mass spectroscopy, radiolabelled cellular assay, and molecular dynamics simulation we demonstrate that betaine has a dual role in GAT1: at mM concentration acts as a slow substrate, and at µM as a temporal blocker of GABA, when it is below its K0.5. Given this unique modulatory characteristic and lack of any harmful side effects, betaine emerges as a promising neuromodulator of the inhibitory pathways improving GABA homeostasis via GAT1, thereby conferring neuroprotection against excitotoxicity. Supplementary Information The online version contains supplementary material available at 10.1007/s00018-024-05309-w.


Introduction
Betaine (N, N, N trimethylglycine) is a small molecule, found in diverse organisms from bacteria and plants to animals.It is a natural, stable, and nontoxic substance that can be produced endogenously in mitochondria by the oxidation of choline [1] and exogenously absorbed as a dietary nutrient from the betaine-rich food sources like beetroot, spinach, and different seafoods [2,3].In mammals, betaine is known to play two primary physiological roles: an osmolyte that protects the cells against osmotic pressure through osmoregulation, and an active methyl donor that enables the conversion of the toxic metabolite homocysteine into methionine [1].In humans, betaine is mainly found in the liver, kidney, and brain.However, the presence and role of betaine in the brain is poorly understood and remains debated [4].
There has been substantial reporting on the beneficial effects of systemic betaine supplementation in neurodegenerative and neuropsychiatric disorders like Alzheimer's [5][6][7], Parkinson's [8], schizophrenia [9], anhedonia [10], and others [4,11,12].This reported evidence implies a role of betaine with a therapeutic potential in the central nervous system (CNS) [4,13].While the evidence for the effects of betaine on neuronal disorders is strong, the cellular and molecular mechanisms involved in its membrane translocation remain unclear.
The solute carrier (SLC) membrane transporters regulate essential physiological functions like nutrient uptake, waste removal, and ion transport.This second-largest family of membrane proteins has much relevance to pharmacology as drug targets or mediators [14].Betaine can enter the brain by crossing the blood-brain barrier (BBB) using betaine/γaminobutyric acid (GABA) transporter 1 (BGT-1, slc6a12) [15,16].However, the low expression of BGT-1 in the CNS raises questions over its effectiveness in betaine transport into the neurons [17].The same is the case for another transporter called sodium-dependent amino acid transporter 2 (SNAT2, slc38a2), that transports betaine and is expressed at low level in the CNS [18].Interestingly, it has been reported that betaine might interact with the GABAergic pathway beyond BGT-1 and play a role as a signalling ligand in the CNS [19][20][21].To investigate the potential modulatory role of betaine, we studied its interaction with GABA transporter 1 (GAT1, slc6a1) [22].The expression of GAT1 is mainly neuronal, predominantly in the adult frontal cortex, and among all GATs it is the most expressed GAT in the CNS.About 80% of GABA from the synaptic cleft is taken up into presynaptic neurons through GAT1 [23].The modulation of the GABAergic activity via regulation of the GABA homeostasis sustains the excitatory/inhibitory (E/I) balance in the CNS, which is a critical factor in protecting the brain against the excitotoxicity and consequently reducing the risk of neurological and neuropsychiatric diseases [24].
The results reported here unveil a new role of betaine in the E/I balance by showing its important action on GAT1.Here, we demonstrate a new relationship between GABA and betaine by integrating data from electrophysiology: twoelectrode voltage clamp (TEVC) and automated patch clamp (Patchliner™), measurements of radiolabelled efflux assays, liquid chromatography-mass spectroscopy (LC-MS/MS), and molecular dynamics simulations.It is important to underline that the concentrations of the two substances used for many of the experimental approaches are closed to their physiological values, supporting the importance of betaine in regulating GABA homeostasis.

Extracellular betaine perfusion on Xenopus laevis oocytes heterologously expressing rGAT1 induces inward transport currents
Fully grown Xenopus laevis oocytes have a highly efficient biosynthetic apparatus that can perform all the post-translational modifications needed for correct protein targeting and function.We use the microinjection technique to gain the heterologous expression of the protein of interest in Xenopus laevis oocytes [25].BGT-1 is reported to transport betaine and GABA in a concentration-dependent manner, with a higher affinity for GABA than betaine [26,27].The perfusion of betaine (1, 3, 10, 30, 50 mM) on the oocytes expressing rat GAT1 (rGAT1) resulted in concentration-dependent inward transport currents, like canine BGT-1 (cBGT-1) (Fig. 1A-C).The representative traces of these betaineinduced currents, in Fig. 1 A, are comparatively shown with the currents induced by GABA 300 µM, which is the saturating concentration for GAT1 in X. laevis expression system [28][29][30].
At the holding potential V h = −60 mV, the kinetic analysis of these inward transport currents provided a halfmaximal transport coefficient K 0.5 = 11.57± 1.78 mM, the maximal transport current I max = −76.15± 3.46 nA, and the transport efficiency I max /K 0.5 = −6.58± 0.80 nA/mM (Table in Fig. 1).As a negative control, the non-injected oocytes were perfused with the same concentrations of betaine.The oocytes expressing rGAT1 and the non-injected control oocytes were also exposed to glycine (from 1 to 50 mM), and in both cases no inward current was observed (Fig. S1A).Additionally, also in Chinese hamster ovary (CHO) cells overexpressing human GAT1 (hGAT1) we recorded a concentration-dependent betaine transport current using the automated whole-cell patch clamp technique (Patchliner™ from Nanion GmbH, Germany) (Fig. S2).

Betaine transport by rGAT1 is sodium-dependent and can be blocked by the inhibitors of GAT1
GAT1 is a sodium-dependent symporter, meaning its transport activity requires a sodium gradient [31].To examine the sodium dependence of betaine induced currents in oocytes expressing rGAT1, after testing them in sodium chloride buffer solution (ND98) we replaced sodium chloride with trimethylammonium chloride (TMA-Cl).The experiments with this buffer solution (TMA98) resulted in the almost complete loss of the GABA-and betaine-induced inward transport currents (Fig. 1D, E).This confirms that like GABA, the betaine transport by rGAT1 also requires sodium.We also tested the effects of SKF89976a (30 µM), a GAT1 inhibitor [32], on betaine transport in the oocytes expressing rGAT1.The presence of SKF89976a in the perfused solutions caused a strong inhibition of the transport current elicited by GABA 300 µM and betaine 10 mM (Fig. 1D, E).Similar effects were also observed with other GAT1 inhibitors tiagabine and NO-711 (Fig. S1B), these data confirm that the betaine-currents are mediated by rGAT1.

The voltage-dependent transport of betaine by GAT1 shows that it is a slower substrate than GABA
GAT1 is a voltage-dependent transporter, and the voltagesteps experiments on X. laevis oocytes expressing rGAT1 reveal pre-steady state, steady-state, and leak currents [33][34][35].The voltage jumps in the presence of betaine (1, 3, 10, 30, 50 mM) performed on the oocytes expressing rGAT1 elicited voltage-dependent transport currents in rGAT1, similar to that induced by GABA [36] (Fig. 2B).
The pre-steady state (PSS) currents in GAT1 are due to the binding and unbinding of Na + to the transporter inside the membrane electric field [37] and usually they disappear in the presence of a saturating concentration of substrate [34].Hence expectedly, at saturating GABA concentration (300 µM), we observed the vanishing of PSS currents as they became too fast to be detected and only the steady state currents were detected (Fig. 2 A, top row).In the presence of SKF89976a (30 µM), the PSS and steady state currents both disappeared (Fig. 2A top row) as this compound blocks the access of Na + to the GAT1 vestibule limiting the translocation of substrate and ions [38,39].The capacitive currents recorded in the presence of the inhibitors are the fast relaxation component due to the membrane capacitance of the oocytes.
Interestingly, even in the presence of increasing betaine concentrations, we observed the persistence of a slow transient component.These relaxations are larger than expected (Fig. 2 A, middle and last row) when compared to that at low GABA concentrations [30].The PSS currents in the presence and absence of betaine were analysed after subtraction from the currents in the presence of SKF89976a 30 µM [25,31] The remainders were integrated to obtain the dislocated charge (Q) and fitted with single exponential to determine the relaxation time constant (τ).The Q-V relationship reflects the charge moved into the membrane electric field at each tested transmembrane potential.Whereas the τ-V relationship provides the rate of the charge dislocation in the transporter vestibule.These data were further analysed to calculate outrate α and inrate β that indicate the rate of charge moving to and from the transporter cavity respectively (Fig. 2C-E) [30,40].All of the Q-V, τ-V, and rate constant analysis were done for betaine 0.1, 0.3, 1, 3, 10, 30, and 50 mM, in the figures the data for betaine 0.1, 1, 10, and 50 mM are reported (for the remaining concentrations Fig. S3).
The Q-V relationship showed that low concentrations of betaine (0.1-1 mM) induced charge displacements similar to ND98 alone (Fig. 2C).With further increase in extracellular betaine (10 and 50 mM) the charge displacement decreased but less than expected and did not disappear like for saturating GABA [30].The τ-V relationship provided a similar result, where the decay time constant decreased with the increase in betaine concentration (Fig. 2D).This indicates an accelerated transport rate in the presence of betaine but again differently from what is known for GABA [30].Further analysis of α and β showed that at low betaine concentrations, the charge entered the transporter cavities faster than it could leave (β > α), similar to the substrate free Na + -buffer solution.Interestingly, β in the presence of betaine 0.1 mM is lower than in the presence of Na + -buffer alone, in particular at voltages lower than −80 mV (Fig. 2E).

Detection of GABA and betaine using LC-MS/MS in X. laevis oocytes expressing rGAT1
While the electrophysiological characterization of the betaine-GAT1 interaction has shown that betaine is a slow substrate of GAT1, we also wanted to detect a direct and voltage-free uptake of betaine by GAT1.In this work, we developed a radiolabelled-free method using a tandem LC-MS/MS based approach to detect the substrates taken up by rGAT1 heterologously expressed in X. laevis oocytes (Fig. 3A).To verify the sensitivity and linearity of the Fig. 2 The pre-steady state analysis of betaine transport by rGAT1.The current response for each condition was collected by giving 0.8 s long squared pulse at -20 mV of from the holding potential of −60 mV, starting from −140 mV to + 40 mV.A The representative traces of the voltage-step response for ND98, GABA 300 µM, SKF89976a 30 µM, and different indicated betaine concentrations.The dashed red line indicates the holding current for the oocyte at the holding potential.B The current and voltage (I-V) relationship from −140 mV to + 40 mV.C The total charge dislocation and voltage (Q-V) relationship.D The decay time constant and voltage (τ-V) relationship.E The relationships of unidirectional rate constants outrate (α) and inrate (β, shown as dashed line) with voltage.All the reported values were collected in the presence of ND98 alone and with betaine 0.1, 1, 10, 50 mM.In C-E the voltage levels tested were from −120 mV to + 20 mV.For B-E, all values are shown as mean ± SEM of 3/1 n/N ◂ LC-MS/MS response to betaine and GABA, standard solutions were created, and a calibration curve was obtained (Fig. S4).The detected retention time for GABA was 1′ 55″ and for betaine 2′ 30″ (Fig. 3).
The oocytes heterologously expressing rGAT1 were incubated in different concentrations of GABA (1, 3, 10, 30, 100, 300 µM) and betaine (0.1, 0.3, 1, 3, 10, 30 mM) for 25 min in groups of five oocytes per sample.For both GABA and betaine, a concentration-dependent uptake by rGAT1 was observed (Fig. 3B, C histogram on right).As a negative control, the non-injected oocytes were also incubated in the same concentrations of GABA and betaine, and their analysis showed an absence of uptake for both substrates.

Both GABA and betaine induce efflux of [ 3 H]-GABA in rGAT1 expressing HEK293 cells
The human embryonic kidney cell line (HEK293) is widely utilized as the platform to express membrane proteins.In the absence of radiolabelled betaine, it was difficult to detect its inward transport in HEK293-rGAT1 cells using uptake assays.In our previous work [41], we demonstrated that We tested the effects of betaine on HEK293-rGAT1 cells pre-loaded with 0.01 µM [ 3 H]GABA at 37 °C for 20 min.The experiment was initiated by replacing the pre-loading buffer with plain Kerbs Ringer HEPES buffer (KHB) and starting the experiment with the collection of baseline efflux values (Fig. 4).Basal [ 3 H]GABA efflux was 0.12 ± 0.02% min −1 .Addition of betaine induced a time-, concentration-, and rGAT1-dependent efflux of [ 3 H]GABA, in the presence and absence of the ionophore monensin (10 µM) (Fig. 4D, E).Monensin (mon) is a sodium ionophore that selectively collapses the Na + and H + gradients, reducing the electrochemical driving force for uptake and favouring the transporter efflux by an increase of sodium inside the cell [42].As a positive control, pre-loaded HEK293-rGAT1 cells were exposed to GABA, and the results matched with the time-, concentration-, and rGAT1-dependent efflux (Fig. 4A,  B), similar to our previous report [41].For kinetic analysis, the drug-induced efflux was calculated as the mean efflux of the fraction where the value started plateauing divided by the length of the fraction (= 2 min).The fitting of the data using non-linear regression by the logistic fitting model provided the parameters as K 0.5,GABA = 36.28± 11.27 µM (with mon 10 µM K 0.5,GABA = 36.48± 2.57 µM) and K 0.5,betaine = 6.73 ± 2.21 mM (with mon 10 µM K 0.5,betaine = 7.71 ± 1.13 mM) (Fig. 4C, F).We also performed a negative control experiment with tiagabine, a GAT1 inhibitor, that resulted in the absence of [ 3 H]-GABA efflux (Fig. 4G).

Molecular dynamics and docking experiments show that betaine binds in the same binding pocket of GAT1 as GABA
Having observed that betaine is a slower substrate of GAT1, with lower affinity than GABA (Figs. 1, 2), we were motivated to understand its binding mechanism with GAT1 using molecular dynamics.In the absence of a crystal or cryo-EM structure of hGAT1 in the outward-facing conformation, we selected the Alphafold homology model to analyse the stability of bound GABA and betaine [37,43,44].The bound ions (two Na + and one Cl − ) were added to the hGAT1 model using as a reference the outward-open human SERT crystal structure (PDB ID: 5I71) [45].The docking studies for betaine to the outward-open hGAT1 provided a successful docking with the best fitness score of 42.24 (Fig. 5A).As a positive control, docking simulations for GABA were also run, which resulted in fitness score of 50.52 (Fig. S5).The carboxyl head of betaine, which overlaps with the carboxyl head of docked GABA, interacts with Na1 (the sodium bound to the NA1 sodium binding site) and formed short-range (d < 3 Å) contacts with the backbone amide protons of L64 and G65, and with the side chain hydroxyl proton of Y140.The tail containing three methyl groups formed two medium-range (3 Å < d < 5 Å) contacts with residues S295 and S396.
Interestingly, the recent work of Zhu et al. assigned five water molecules in GABA binding pocket in hGAT1.They showed in the inward occluded state, the amino acid group of GABA is stabilized by the hydroxyl group of T400 and a water molecule [46].When we overlapped our hGAT1 model with GABA docked in the outward-open state with the inward-occluded cryo-EM structure of hGAT1 with GABA from Zhu et.al. (Fig. 5B), we observed similar stabilization of docked GABA in our model.Moreover, we also performed the same overlapping of the cryo-EM structure by Zhu et.al. with our outward-open hGAT1 with betaine docked (Fig. 5C).This overlapping showed that betaine molecule is not long enough to have a stable polarcontact with T400, but in the presence of a water molecule (stabilized by T400) it can form a stable hydrogen-bond and could allow the conformational change to the inward-open state.
The MD simulations were performed using the three docking poses of betaine with the best fitting scores (Fig. 5D,  E).The simulations were run for 50 ns (the simulation parameters are reported in supplementary information as Code S1) and resulted in betaine stably bound to hGAT1, with root mean square displacement lower than 0.2 nm (Fig. 5F).The simulated GAT1 also resulted in a stable conformation, showing root mean square fluctuations greater than 0.2 nm only in residues belonging to the extracellular and intracellular loops (Fig. 5G).

The relationship of GABA and betaine in rGAT1 depends heavily on their extracellular concentrations
The neuroprotective properties of betaine have been reported in many publications, with a positive correlation with the GABAergic pathway.To determine the mechanism of action betaine with GAT1 and the possible impacts on the GABAergic pathway, we explored its relationship with GABA, the primary substrate of GAT1.We investigated the GABA-betaine relationship using TEVC and LC-MS/ MS.The competitive assay experiments on TEVC were performed using six GABA concentrations ranging from 1 to 300 µM with eleven betaine concentrations from 0.001 to 50 mM.The GABA concentrations chosen to study the GABA betaine relationship are based on the kinetic parameters GABA transport by rGAT1 and hGAT1 obtained for and reported in the literature [29,30,47,48].The representative traces of the currents collected in the competitive assay at the holding potential of −60 mV are reported in Fig. 6A.With GABA concentration below 10 µM and betaine below 10 mM, we observed a reduction of the total transport current indicating an inhibition of the GABA transport.With betaine 10 mM and above, this blocking effect disappeared, and a collective larger inward transport current was observed.The mean values of the currents for all 84 conditions are reported as a heat map of GABA-betaine competition (Data available in Table S3).The data showed that the GABA-betaine relationship starkly depends on their individual extracellular concentration (Fig. 6B).
Since in our LC-MS/MS protocol the detection time for GABA and betaine uptake by rGAT1 are different and have distinct production-ions, it was possible to use this method to perform GABA and betaine competition in the same oocyte.Based on the electrophysiological findings, the inhibitory effect of betaine on GABA transport was the most at 0.1 mM concentration.Therefore, we incubated the oocytes expressing rGAT1 with GABA 3, 10, and 30 µM with betaine 0.1 mM for 25 min (n = 3, five oocytes per sample).The cytosolic contents detection by LC-MS/ MS for the uptake of all three GABA concentrations were compared with and without betaine 0.1 mM (Fig. 6C).The histogram showed that in the presence of betaine 0.1 mM: with GABA 3 µM no GABA was taken up, with In C: inward-occluded in red), betaine and GABA shown as sticks, and Na + (purple) and Cl − (green) as spheres GABA 10 µM the GABA uptake was significantly reduced, and with GABA 30 µM the GABA uptake didn't alter significantly.
Taken together, these data showed that betaine has a dual effect on GABA transport by rGAT1.This duality can be best visualized at GABA 10 µM with different betaine concentrations (Fig. 6D).When GABA 10 µM is co-applied with betaine from 1 to 300 µM, concentration-dependent inhibition of GABA 10 µM transport current was observed.At the same GABA concentration, the perfusion with betaine from 1 to 50 mM yielded a concentration-dependent increase in transport current.This kind of dual effect of betaine on GABA transport vanished when the extracellular GABA concentration was 30, 100, and 300 µM i.e., larger than K 0.5,GABA .

Betaine slows down the GAT1 transport cycle inhibiting GABA uptake
The competition experiment of GABA and betaine was also performed with the voltage-steps protocol to study the steady and PSS transport currents.By observing the representative traces in the presence of GABA 10 µM with and without betaine 0.1 mM, the peculiar inhibitory action of betaine is visible.We observed a reduction in the current amplitude (indicated by the red dotted line) and increment in the decay time of the PSS currents in response to the voltage jumps (Fig. 7A).The I-V relationship for GABA 10 µM in the absence and presence of betaine 0.1 mM revealed the apparent blocking effect of betaine (Fig. 7B).Also, the Q-V analysis showed that in the presence of betaine 0.1 mM, the total charge dislocated by GAT1 did not increase significantly than of GABA 10 µM alone (Fig. 7C).While the τ-V relationship for low betaine concentration (0.1 mM) (Fig. 2) showed an overall similar decay time constant as ND98, whereas for low GABA concentration (10 µM) the decay time constant was much faster (Fig. 7D).Interestingly, τ for GABA 10 µM with betaine 0.1 mM, slowed down significantly, especially at the positive transmembrane potentials (Fig. 7D), indicating slowing down of the transport cycle.Similarly, both decay constants, α and β for GABA 10 µM in the presence of betaine 0.1 mM, showed an overall reduction, significantly in α at the positive transmembrane potentials (Fig. 7E).Altogether, it is evident that in the presence of betaine the transport rate of GAT1 for GABA decreased.

Discussion
Betaine is an endogenous molecule that plays an essential dual role as an osmolyte and a methyl donor in human physiology.In the past few decades, several studies have reported the beneficial effects of betaine in neurological and neurodegenerative diseases, however, the mechanism of its action at the cellular and molecular level remained unclear.Its systematic supplementation showed only mild side effects [4,49,50], making it a therapeutic molecule of interest.However, the presence of betaine in the brain and the mechanism involved leading to its positive action still remained a puzzle, deeming it a "dark knight" [4].
In this work, we show that betaine can be transported in a concentration-dependent manner by the most expressed neuronal GABA transporter GAT1, and that betaine modulates the uptake of GABA.From this data, we infer that betaine can modulate the extracellular GABA concentration and play a role in maintaining the E/I balance in the CNS.
In humans, mitochondria can produce betaine in small quantities, but the primary source is the oral uptake from the dietary sources [1,51].As betaine is an excellent osmolyte, it tends to get accumulated in cells and tissues [52], leading to the underestimation of betaine absorption when using the traditional blood plasma assays [53,54].The pharmacokinetics of this accumulation is dose-dependent with the peak betaine concentration reaching 1-3 mM within hours after intake [55,56].In liver and kidney, the concentration of betaine can reach up to ~ 30 mM and ~ 100 mM respectively [4,57].The reported betaine level in the mice brain is unclear [58], although recently Knight et al. showed that the neurons from the hippocampal tissues of mice, can uptake and accumulate betaine up to 12 mM [54].From their findings, it is conceivable that the neuronal concentrations of betaine might reach millimolar levels.With this argument along with the fact that the affinity of betaine for BGT-1 also ranges towards millimolar [26], we used betaine at millimolar levels to study its interaction with GAT1 and BGT-1.Moreover, the physiological concentration of GABA in the CNS ranges between 0.1-1 mM [59,60].Thus, the chosen concentrations for both GABA and betaine in this work correspond to their reported physiological values, making the data shown physiologically relevant.
The electrophysiological measurements using TEVC in X. laevis oocytes heterologously expressing rGAT1 resulted in betaine-induced concentration-, voltage-, and sodium-dependent inward transport currents, which could be inhibited by GAT1 inhibitors like SKF89976a (Fig. 1), tiagabine, and NO-711 (Fig. S1).The transport of betaine by GAT1 was also confirmed with automated patch-clamp (using the Patchliner™) on CHO cells overexpressing hGAT1 at V h = −80 mV with EC 50 ≈ 27 mM (Fig. S1).We also showed betaine translocation by GAT1 using radiolabelled efflux assay in HEK293 cells and LC-MS/MS analysis of the cytosol contents of X. laevis oocytes (Figs. 3  and 4).
The kinetic analysis of the GABA and betaine transport currents in GAT1 and BGT-1 reveals something interesting (Table in Fig. 1).For GABA, the transporter efficiency (I max /K 0.5 ) of GAT1 is about ten times larger than BGT-1, meaning that GAT1 can transport a lot more GABA than BGT-1.Whereas, for betaine, the transporter efficiency of GAT1 is almost 0.5 times less than BGT-1.This suggests that compared to GABA there is little difference between the amount of betaine that can be transported by GAT1 and BGT-1.Thus, BGT-1 cannot transport GABA efficiently like GAT1, but GAT1 can transport betaine with efficiency close to that of BGT-1.
The detailed analysis of the PSS currents gives information about the initial steps of the transporter cycle and the interaction of the transporter with ions and substrate [22].The analysis of the decay time constant (τ) of the large transient currents as outrate α and inrate β constants showed that in the presence of betaine (0.1 and 1 mM), β of rGAT1 increased.This implies that when betaine is present at low concentration and binds in the GAT1 vestibule, it cannot induce the same fast conformational changes, as GABA [38].Also, the higher inrate than the outrate of charge dislocation suggests that in the presence of betaine, especially at lower concentrations, the transporter cannot transit to the inwardopen state as fast as in the presence of GABA.This behaviour of GAT1 suggests that it requires a third "interaction" to transport betaine as in BGT-1 [26] or that the conformational transition towards the inward open state is less efficient.This is further supported by the Q-V relationship of betaine in GAT1, where the curve is shifted towards more positive voltage (for 0.1 mM betaine: V 0.5 = −27.16± 2.57 mV, voltage where half of the charge is moved) than for GABA (for GABA 10 µM V 0.5 = −43.19± 3.38 mV) and ND98 alone (V 0.5 = −32.87± 1.10 mV) (Fig. 7C and Table S1).Interestingly, a similar shift in V 0.5 , could also occur when the extracellular Na + concentration is changed [31].In the experiments reported here, extracellular Na + concentrations were unaltered, consequently, this shift can be related to either an apparent change in Na + concentration inside the transporter vestibule or a decrease of the Na + dissociation [56].Moreover, the molecular docking and MD simulations of betaine-bound hGAT1 showed that it forms less shortrange contacts than GABA (Figs. 5A, S5).This implies that it would require involvement of more residues to stabilize the binding of betaine than GABA, suggesting it as a factor behind the lower affinity for betaine in GAT1.In summary, the transition of GAT1 out of the occluded state is slower for betaine than GABA, but it might not be the only possible interpretation of our data.
The GABA-betaine competitive assay experiments clearly showed that their relationship is strongly concentrationdependent (Fig. 6).At the high physiological GABA concentrations, betaine shows minimal impact on the GABA transport by GAT1.In contrast, when the extracellular GABA concentration is lower than its physiological K 0.5 (≈16 µM), betaine at concentrations of 0.1-3 mM inhibits GABA transport by GAT1.It is important to note that the concentration of GABA and betaine that gave rise to this peculiar phenomena are in the range of the values reported as physiological concentrations in human brain [54-56, 59, 60].The reduction of the transport rate in the presence of betaine has a role in this selective inhibition of GABA transport.In the presence of low extracellular betaine, both the inrate and outrate of GABA reduced starkly (Fig. 7D, E and Table S2).As the time required for betaine to be moved inside the cell is longer than GABA, the betaine remains bound to some of the GAT1 proteins, reducing the available transporters able to complete the cycle in the presence of GABA lower than K 0.5,GABA .Consequently, several transporters fail in rapid completion of their cycle, enabling the modulation of the GABA uptake by betaine.When the concentration of GABA reaches close to the saturation, it outcompetes betaine allowing rapid completion of the transport cycle.While at high concentrations (> K 0.5,betaine ), betaine behaves like a regular substrate as the higher chemical gradient provides energy for its slower intracellular translocation by GAT1.This inhibitory role of betaine was also confirmed by LC-MS/MS, which showed that the uptake of extracellular GABA, when < K 0.5,GABA , was significantly reduced by betaine 0.1 mM (Fig. 6C).This kind of selective inhibition by betaine appears to be specific to GAT1 and was not observed in BGT-1 (Fig. S6).Also interestingly, betaine did not show any selective inhibition of the nipecotic acid (another GAT1 substrate) induced transport currents in GAT1 (Fig. S7).
The conventional GAT1 blockers derived from its competitive inhibitor nipecotic acid were modified with lipophilic sidechains to allow the blood-brain barrier (BBB) penetration and disable the substrate properties [61,62].One such derivative, tiagabine, which is the only anticonvulsant drug targeting GAT1, is used to treat partial seizures in patients with epilepsy.However, tiagabine treatment has been reported to cause several unwanted side effects such as confusion, abnormal mood swings, dizziness, tremors, fatigue, and nervousness [63].The recent works on GAT1 structures suggest that tiagabine may bind GAT1 in the outward open conformation and blocks in the inward open conformation, disabling any further uptake by the transporter [38,39,46,64].Differently from tiagabine, betaine slows down the transport cycle of GAT1 and triggers a temporal inhibition of GABA uptake.This effect can be abrogated by the increase of extracellular GABA, which will allow the transporter to regain its original function of the GABA uptake.Along with this unique blocking characteristic and the minimal harmful side-effects associated with its supplementation, betaine could be a useful molecule to modulate GABA homeostasis targeting GAT1.
Importantly, betaine does not require chemical modifications to cross the BBB.Wang et al. showed in vivo that the cylindrical polymer brushes (CPB) modified with betaine could cross the BBB [65].They also performed in vitro uptake experiments on endothelial bEnd.3 cells to identify the transport mechanism for the modified CPBs and deemed BGT-1 as the transporter responsible for the translocation.Interestingly, the uptake inhibition of the modified CPB by GABA was much stronger than by betaine, which they correlated with the higher affinity of BGT-1 for GABA than betaine.By taking in account our results of betaine transport by GAT1, it would suggest that along with BGT-1, also GAT1, which is expressed in bEnd.3 cells [66], could have contributed to the translocation of the modified CPBs.
The E/I balance in the CNS is essential for the healthy, stable, and physiologically functional neuronal circuits; and the disruption of this balance is the primary cause of many neurological diseases [67].Given that GABA is the primary inhibitory neurotransmitter in the CNS, its homeostasis is essential for the formation of learning and memory.The systematic supplementation of betaine has been shown to ameliorate the E/I balance-related diseases such as Alzheimer's, Parkinson's, dementia, schizophrenia, and stress-related disorders, but these results lack substantial mechanistic explanation [4].Since the extracellular GABA levels are critical for these disorders and diseases, the peculiar GABA inhibitory behaviour of betaine can explain its beneficiary effects from the molecular point of view.
Recently Knight et al. showed that the hippocampal neurons not only uptake and accumulate betaine, but also modulate the neuronal uptake of other essential osmolytes in response to the changes in osmolarity [54].Especially under hyperosmotic conditions, hippocampal neurons preferentially uptake betaine over glycine and glutamine.This connects neuronal uptake of betaine with glycine, an essential inhibitory neurotransmitter, and glutamine that is the precursor to the production of both glutamate (the primary excitatory neurotransmitter) an GABA (the primary inhibitory neurotransmitter).Such interaction of betaine with different essential elements of neurophysiological processes suggests its participation in more than one [68].Especially, with the GABA inhibitory behaviour of betaine shown here suggests a possibly larger modulatory role of betaine in maintaining the E/I balance in the CNS.
Moreover, it was shown by Hardege et al. that the Caenorhabditis elegans nervous system can synthesize betaine, specifically in the interneurons, and use it as a modulator of different behavioural states [21].They also showed that the vesicular transporter CAT-1 expressed in the interneurons could transport betaine, suggesting nematode neurons can load betaine in the synaptic vesicles.Lastly, the work from Kunisawa et al. showed that the lack of betaine in rats could affect GABAergic transmission and memory formation [19].They also demonstrated that these effects of betaine are regulated not solely by BGT-1 but partly mediated by betaine modulating the GABAergic system.These results along with the data presented here, strongly suggest that betaine should have a specific role in the CNS (possibly a neuromodulator) apart from being an osmoregulator and a methyl donor.
As GABA is the primary inhibitory neurotransmitter in the CNS, it plays a major role in the regulation of E/I balance.GATs are responsible for the clearance of GABA from the synapse, they contribute significantly to maintaining the E/I balance playing a role in E/I balancerelated neurological and neuropsychiatric disorders [22,67,69].Suñol et al. showed the synergic anticonvulsant effects of GAT1 selective inhibitor tiagabine and the BGT-1 selective inhibitor EF1502 [70].They highlighted that BGT-1 could also have a functional role in GABA clearance suggesting a role in controlling epileptogenic effects.Interestingly, Fuehrer et al. showed that in AD patients there is a significant upregulation of BGT-1 in the superior temporal gyrus, whereas GAT1 expression decreases [71].As betaine has shown to ameliorate conditions in AD by acting against the oxidative stress induced by generation and deposition of amyloid-β and toxic homocysteine, this kind of upregulation of BGT-1 could be a response to the increased oxidative and osmotic stress during AD [71][72][73].Considering our results demonstrating the neuromodulatory action of betaine via GAT1, it is possible that in neurodegenerative diseases that cause loss of neurons, like AD and PD, betaine could benefit not only by protecting the CNS against oxidative stress, but also by regulating GABA levels to maintain the E/I balance.
Overall, this work confirms the betaine transport by GAT1 and the concentration-dependent modulation of GABA transport by GAT1 using betaine.Naturally, these findings raise the question of whether other neurotransmitter transporters and receptors may interact with betaine.While our work answers one of the questions around the role of betaine, it is now even more important to explore its presence and investigate its effects in the brain, beyond being a substrate of BGT-1.Betaine carries the potential of being a natural neurotherapeutic agent and given its already an FDA-approved drug (Cystadane® for homocystinuria), it would be of great interest to explore its applications in the clinical trials of GABAergic drug as a natural neuroprotective agent.
Human embryonic kidney 293 (HEK293) cells stably expressing the rat isoform of GAT1 (rGAT1) were used (rGAT1-HEK293 cells) in batch release assays.The generation and maintenance of stable cell lines expressing rGAT1 was conducted as previously described by other for other SLC6 transporters [74].rGAT1-HEK293 cells were maintained in high glucose (4.5 g/L) and l-glutamine- containing DMEM, supplemented with 10% FBS and G418 (250 µg/mL) in a humidified atmosphere (37 °C, 5% CO 2 ) and in a sub-confluent state.

Heterologous expression in X. laevis oocytes
The detailed experimental procedure has been described elsewhere [76].Briefly, the cDNAs encoding rat GAT1 in the pAMV vector, and Madin-Darby canine kidney (MDCK) canine BGT-1 in the pSPORT1 vector were linearized using NotI, and the in vitro cRNA synthesis was done in the presence of Cap Analog 10 mM and T7 RNA polymerase 200 U.
Oocytes were collected from X. laevis female frogs, under anaesthesia, by performing laparotomy on the abdomen, to remove portions of the ovary.Detailed procedures are described elsewhere [25].For the heterologous expression of the GABA transporters, stage IV oocytes were micro-injected with cRNA encoding the target protein i.e., rGAT1 and cBGT-1 (12.5 ng/50 nL) and incubated for the expression period (3)(4)

Electrophysiology
The two-electrode voltage clamp (TEVC) Oocyte ClampOC-725B, Warner Instruments, Hamden, CT, USA was used for controlling voltages and recording currents.The clamped oocytes were maintained under continuous perfusion of the basic buffer solution ND98 (NaCl 98 mM, CaCl 2 1.8 mM, MgCl 2 1 mM, HEPES 5 mM at pH7.6) with a flow rate of 1.5 mL/min.For concentration -response curves and competitive assay experiments, solution exchange was performed using an in-house developed gravity-driven digitally controlled perfusion control system.Signals were filtered at 0.1 kHz and sampled at 1 kHz.The voltage-step experiments were performed by the voltage pulse control protocol consisting of 10 square pulses (0.8 s long) from -140 mV to + 40 mV (at 20 mV increments).All recorded currents were digitalized using Axon CNS 1440B Digidata system controlled by pClamp 11.2.2 (Molecular Devices, USA).
For whole-cell patch clamp experiments using CHO cells expressing human GAT1 on the Patchliner™ (Nanion Technologies GmbH, Germany), the cell-harvesting was performed right after the setup of the instrument, to be transferred directly into the CellHotel™.The cells were automatically transferred from the CellHotel™ to each of the eight wells of 4X chips for Patchliner™ that was set in the whole-cell mode with the holding membrane potential at −80 mV.
The internal solution (10 mM NaCl, 110 mM KF, 10 mM EGTA, 10 mM KCl, and 10 mM HEPES at pH 7.2) was provided inside the cells, followed by the external solution outside (Ca +2 -rich, 130 mM NaCl, 4 mM KCl, 10 mM CaCl 2 , 1 mM MgCl 2 , 5 mM d-Glucose monohydrate, 10 mM HEPES at pH 7.4) for seal enhancement.For the recording on the Patchliner™, only cells showing a seal resistance > 300 MΩ were taken into consideration for the analysis.After the seal was established, a double wash with external solution (standard, 140 mM NaCl, 4 mM KCl, 2 mM CaCl 2 , 1 mM MgCl 2 , 5 mM d-Glucose monohydrate, 10 mM HEPES at pH 7.4) was performed to remove the extra Ca 2+ .The following fluidic protocol was followed for all betaine concentrations: 6 s perfusion of 60 µL of betainecontaining external solution (speed 10 µL/s) followed by 18 s perfusion of 180 µL of external solution (standard) to wash away the betaine (speed 10 µL/s).

Substrate detection in X. laevis oocytes using LC-MS/MS
To perform the substrate uptake experiment, the X. laevis oocytes expressing rGAT1 were incubated in a fresh Petri dish containing the substrate + ND98 for 25-30 min at 18 °C.To remove any presence of the extracellular substrate post-incubation, the oocytes were carefully washed thrice with ice-cold ND96 for two minutes.At the end of the washing, the oocytes (in the group of 5) were transferred in a fresh Eppendorf containing CH 3 OH:CHCl 3 :H 2 O in proportion of 3:1:1 v/v with the solvent to oocytes ratio of 1:100.The oocytes were homogenized using water ultrasonicator and then centrifuged at 13,000xg for eight minutes at 4 °C.The supernatant from these samples was removed, and the pallet containing the cytosol content with oocyte debris were diluted in H 2 O (MilliQ, Merck, Italy) to extract the hydrophilic compounds.These samples were centrifuged at 13,000xg for eight minutes at 4 °C and the aqueous top part containing cytosol content was extracted and used immediately for LC-MS/MS detection or stored at −80 °C to use later (up to three months).
Betaine and GABA standard stock solutions (1 mM in 0.1% formic acid) were prepared in MS grade water.For quantitative mass spectrometry, a Finnigan LXQ linear ion trap mass spectrometer, equipped with an ESI ion source (Thermo Electron Corporation, CA, USA) was used.The analyses were performed in positive (spray voltage 4.5 kV, capillary temperature 270 °C) and in the multiple-reaction monitoring (MRM) mode.The tuning parameters, the optimization of collision energy for each substance, and the choice of target compound fragments were conducted in continuous flow mode by using standard solutions at a concentration of 5 μM.The MRM acquisitions for GABA and betaine were accomplished by monitoring the 114/89 and 118/59 transitions, respectively.The HPLC analysis was performed using a Finnigan Surveyor MS plus HPLC system (Thermo Electron Corporation, CA, USA).For both GABA and betaine quantitation, separation was achieved using the C18 column (ACQUITY UPLC Peptide BEH C18 Column, 300 Å, 1.7 µm, 2.1 mm × 150 mm).The mobile phase was composed of (A) water with 0.1% (v/v) formic acid and (B) acetonitrile (100%) plus 0.1% (v/v) formic acid with a flow rate 200 µL/min; gradient 0-7.0 min/2% (v/v) B, 7-10 min/2-50% (v/v) B; 10-15 min/50-2% (v/v) B.
To verify the sensitivity and linearity of the LC-MS/ MS response to GABA and betaine, calibration curves showing the relative peak areas plotted against analytes concentrations (range 2-16 µM) were created.GABA and betaine contents were expressed as relative intensities (peak areas) among samples.

Radiolabelled GABA release assay
The batch-release assays have been conducted as described before [77,78].In brief, the transfected HEK293 cells overexpressing rGAT1 were grown overnight onto polyd-lysine coated 96-well plates (4 × 10 4 cells/well).After removing DMEM, the cells were loaded with 0.01 µM [ 3 H]-GABA in Krebs-Ringer HEPES buffer (KHB; NaCl 120 mM, KCl 3 mM, CaCl 2 2 mM, MgCl 2 2 mM, glucose 20 mM, HEPES 10 mM at pH 7.3) for 20 min (5% CO 2 , 37 °C).After the incubation, the cells were brought to room temperature and washed five times with KHB during 15 min.Afterwards, cells were kept during 10 min either in KHB or KHB + monensin (mon) 10 μM and the resulting supernatant was discarded.The batch-release assay started by applying either KHB or KHB + mon 10 μM (100 μL; every 2 min, four times).Subsequently, the substance of the interest (in KHB or KHB + mon 10 μM) was added at a specific concentration (every 2 min, five times).The resulting supernatants were collected and transferred to the neighbour wells.Tiagabine (10 μM) and GABA (1-300 μM) were used as negative and positive controls, respectively.Three independent experiments were performed in duplicate for every compound and respective concentration of interest.At the end, liquid scintillation cocktail was added to the wells with remaining cells, with transferred supernatant and to the wells used for total uptake and activity measurements.The total radioactivity present in the supernatant and in the remaining cells was set as 100%, and the amount of [ 3 H]-GABA present in the supernatant was expressed as percentage of the total.

Molecular docking and molecular dynamics simulations
In the absence of a crystal or cryo-EM structure of GAT1 in the outward-facing conformation, we selected the Alphafold homology model to analyse the stability of the docked and bound betaine [43,44].The docking experiments were performed using GOLDscore scoring function on GOLD molecular docking software (The Cambridge Crystallographic Data Centre, UK).For MD simulations, the bound-ions were added to the GAT1 model using the outward-open human SERT crystal structure (PDB ID: 5I71) [45] as a reference.The generated system was converted from full-atom into a coarse grain representation using the MARTINI force field [79][80][81], with a membrane composition of 1-palmitoyl-2-oleoyl phosphatidylcholine (POPC): cholesterol containing membrane (POPC:CHOL 70:30 mol%) [82] solvated in water with 150 mM NaCl.After 1 μs of coarse-grain simulation, while restraining the protein structure, the membrane was equilibrated.The coarse-grained system was then converted to an all-atom representation [83] in which the transporter was replaced by the original GAT1 model to avoid factitious structural imprecisions induced by the double coordinate conversion of the protocol.Betaine was positioned according to the docking results.Possible atom overlaps between the reinserted protein and the relaxed membrane were loosened using the membed procedure [84] as previously described [85].We used the amber ff99SB-ILDN force field [86] to describe GAT1, ions and the solvent, and Slipid [87] for POPC and cholesterol.Previously reported structural analysis of the orthologous SERT structure [45], suggests that the residue E467 is protonated.All simulations were carried out with GROMACS version 2021.4 [88].Three replicas of the final assembled system were energyminimised and equilibrated in four steps of 2.5 ns, each by stepwise releasing the position restraints (1,000, 100, 10, 1 kJ/mol/nm) that are active on the Cα atoms and the bound chloride ion [89,90].Per each trajectory, the production run was carried for 500 ns after removing all position restraints.The temperature was maintained at 310 K using the v-rescale (τ = 0.5 ps) thermostat [91], while separately coupling protein, membrane, and solvent.The pressure was maintained at 1 bar using the Parrinello-Rahman barostat [92] in a semi-isotropic manner and applying a coupling constant of 20.1 ps.Long-range electrostatic interactions were described using the smooth particle mesh Ewald method [93] applying a cutoff of 0.9 nm.The van der Waals interactions were described using the Lennard Jones potentials applying a cutoff of 0.9 nm.Longrange corrections for energy and pressure were applied.Coordinates of all atoms were recorded every 5 ps.The complete set of parameters of the production run can be found in the supplementary materials (Code S1).

Electrophysiological analysis
For TEVC, data analysis was performed using Clampfit 11.2 (Molecular Devices, USA).The dose-response currents were calculated as the maximum current amplitude during the perfusion, and the curves were fitted by nonlinear regression to the Logistic equation using Originpro 8 (OriginLab Corporation, USA).The pre-steady state currents in rGAT1 were isolated by subtraction of the corresponding trace in the presence of SKF89976a 30 µM, as this molecule blocks all of the transport-associated steady state and transient currents [29,30].The resultant traces were fitted with single exponentials to obtain decay time constant and voltage (τ-V) curves.The same traces were used to obtain the charge dislocation-voltage (Q-V) curves by fitting with Boltzmann equation to the sigmoidal curve, which also provided maximal displaceable charge Q max [30,40].The further derivation of τ-V and Q-V curves yielded the unidirectional rate constants inrate (α) and outrate (β) (Eq.1).Equation 1: The Boltzmann equation quantifies Q in , total displaced charge.Where Q max is the maximal displaceable charge, V 0.5 is the voltage at which half maximal charge is displaced (i.e., midpoint of the sigmoidal), σ represents the slope factor.The inrate and outrate constants provide the unidirectional constants α and β respectively.
The data collected with Patchliner™ were saved as ASCII files and successively analysed with the software OriginPro 2021 (OriginLab Corporation, USA).The traces were filtered (using a weighted Adjacent-Averaging filter with ten points of window) and for each cell the baseline was subtracted to the respective betaine traces.The transport current was read as average ± SD (standard deviation) of the current value between 4 and 6 s after betaine perfusion.It is to be noticed that the current in each well is generated by the sum of currents coming from four cells simultaneously since each well of a 4X chip contains four holes for cell attachment.

Fig. 1
Fig. 1 Betaine induces concentration-and sodium-dependent inward currents in Xenopus laevis oocytes expressing rGAT1, which can be blocked by SKF89976a.A Representative traces of current recorded for GABA 300 µM and increasing betaine concentration (0.3-10 mM) in non-injected control oocytes, oocytes expressing cBGT-1, and rGAT1 (top to down).B A violin scattered plot shows the concentration-dependent response of betaine (0.1-50 mM) in rGAT1.The current values are shown as mean ± SEM of 21/5 n (number of oocytes)/N (number of batches).C The kinetic analysis of the betaine transport in rGAT1 yielded I max = −76.16± 1.12 nA, K 0.5 = 11.57± 1.28 mM, (see Table).In the inset, for cBGT-1 the

Fig. 3
Fig. 3 Detection of GABA and betaine transport by rGAT1 using the LC-MS/MS protocol on X. laevis oocytes.A A cartoon of the protocol developed to extract the cytosol contents of the oocytes and detect the presence of the substrate of interest.B A representative trace showing the presence of GABA in rGAT1 expressing oocytes incubated in GABA 1 mM.The histogram on the right shows a qualitative measurement of a concentration-dependent GABA uptake by rGAT1 expressing oocytes incubated in different GABA concentrations (1-300 µM).C A representative trace showing the

Fig. 4
Fig. 4 Betaine induces efflux of [ 3 H]-GABA in pre-loaded HEK293 cells overexpressing rGAT1.A Time course of the efflux of [ 3 H]-GABA in the presence of increasing GABA concentrations (1-300 µM).B Time course of the efflux of [ 3 H]-GABA in the presence of monensin 10 µM and different GABA concentrations (1-300 µM).C The kinetic analysis of the [ 3 H]-GABA-induced efflux with and without monensin 10 µM.D Time course of the efflux of [ 3 H]-GABA in the presence of different betaine concentrations (1-100 mM).E Time course of the efflux of [ 3 H]-GABA in the

Fig. 5
Fig. 5 Molecular docking and MD simulation of betaine and GABA in hGAT1 show that betaine stably binds to GAT1 and forms less polar contacts than GABA.A The successful docking of betaine in hGAT1 with zoomed-in view of the binding site.B The overlapping of GABA-bound hGAT1 Alphafold in outwardopen (in white) with cryo-Em structure of the hGAT1 in the inward-occluded (PDB: 7Y7W, in red) with zoomed-in view of the GABA binding site, in the presence of water molecule stabilized by T400 shown in yellow dashed line.C The same overlapping for betaine-bound structure shows the tail of betaine forming hydrogen-bond with water molecule that is stabilized by carboxyl head of T400 shown in yellow dashed line.D MD simulation results for hGAT1 in the outward open conformation bound to betaine is with a zoomed-in view as the S1-site.The average occupancy from three simulations is visualized using an isosurface, color-coded according to the legend.E The docking poses (in white) and the respective end structures (in light red) at 50 ns resulting from MD simulations.F The root mean square displacement of each replica smoothened with a running average over 2 ns.G.The root mean square fluctuation of hGAT1 residues by plotting a mean root mean square fluctuations value from the three replicas, emphasizing residues belonging to TM helices with a grey bar.In panel A, the short-range contacts (d < 3 Å) are indicated as red dashed lines and mediumrange contacts (3 Å < d < 5 Å) as yellow dashed lines.The representation illustrated includes hGAT1 as ribbons (in A-D: outward-open in white.In C: inward-occluded in red), betaine and GABA shown as sticks, and Na + (purple) and Cl − (green) as spheres

Fig. 6
Fig.6 Betaine has a dual role in rGAT1, a GABA inhibitor at low concentrations and a secondary substrate at higher concentrations.A Representative traces of GABA betaine assay in X. laevis oocytes expressing rGAT1 at holding potential V h = − 60 mV, where the oocyte was perfused with different GABA concentrations (1, 3, 10, 30, 100 μM) along with betaine 0.1, 1, and 10 mM.B The heatmap analysis of the GABA betaine competitive assay shows their concentration-dependent relationship, using the combination of GABA (1-300 μM) with betaine (0.001-50 mM).Data are shown as mean ± SEM of 6/2 n/N.C Detection of GABA and betaine in the oocytes incubated in GABA 3, 10, 30 µM with betaine 0.1 mM, using LC-MS/MS protocol.The qualitative analysis of GABA and betaine uptake by the oocytes is represented in this bar plot with

Fig. 7
Fig. 7 Betaine inhibits the GABA uptake by slowing down the transport cycle of rGAT1.A The representative traces of the voltagestep response, from −140 mV to + 40 mV of the oocyte expressing rGAT1, at holding potential V h = −60 mV, with non-saturating GABA 10 μM (left) and GABA 10 μM + betaine 0.1 mM (right), the dashed red line indicates the holding current for the oocyte at the holding potential.B The current and voltage relationship of GABA 10 μM alone and with betaine 0.1 mM, from −120 mV to + 20 mV, shows the transport current reduction at all voltages.C The total charge dislocation and voltage relationship of GABA 10 μM alone and with betaine 0.1 mM, from −120 mV to + 20 mV shows more charge dislocation happening in the presence of betaine.D The days) at 18 °C before the experimental procedure.The oocytes used in this work were either bought from EcoCyte Bioscience GmbH, Germany or donated by a collaborator with approved experimental protocol by the Committee of the "Organismo Preposto al Benessere Animale" of the University of Insubria, Varese, Italy, and nationally by Ministero della Salute (n.449/2021-PR), Italy; and used in agreement with the Art.18 of decreto legislativo 4 marzo 2014, n. 26 and Art.26 in directive 2010/63/eu of the European parliament and of the council of 22 September 2010.