Functional Characterization of Two Novel Mammalian Electrogenic Proton-dependent Amino Acid Cotransporters

Boll, Michael; Foltz, Martin; Rubio‐Aliaga, Isabel; Kottra, Gábor; Daniel, Hannelore

doi:10.1074/jbc.m200374200

Cited by 154 publications

(241 citation statements)

References 24 publications

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“…They have an exceptional position among the mammalian amino acid transporters, as they act as electrogenic amino acid/proton symporters. Transport is dependent on the extracellular pH, but is independent of sodium, chloride, and potassium ions [1,2,4,7]. Moreover, PAT1 and PAT2 mediated amino acid influx leads to a pronounced intracellular acidification [2,9] by cotransport of the zwitterionic amino acid substrates and protons with a stoichiometric coupling of 1 : 1 as shown for the model substrate L-proline [2].…”

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“…Moreover, PAT1 and PAT2 mediated amino acid influx leads to a pronounced intracellular acidification [2,9] by cotransport of the zwitterionic amino acid substrates and protons with a stoichiometric coupling of 1 : 1 as shown for the model substrate L-proline [2]. Substrates of both transporters are the small apolar amino acids glycine, L-alanine, and L-proline [1,2,[4][5][6][7][8]. Besides these common functional properties, distinct differences became obvious within substrate recognition and electrophysiological characteristics of the two transporters.…”

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“…Whereas substrate affinity is dependent on extracellular pH, proton binding affinity to PAT2 is substrate-independent, favouring a sequential binding of proton followed by substrate. Maximal transport currents are substrate-dependent which suggests that the translocation of the loaded carrier to the internal side is the rate-limiting step.Keywords: electrophysiology; functional characterization; proton symporter; substrate recognition; transport mode.The proton/amino acid transporter family PAT (SLC36) has been identified from human, mouse and rat origin during the last three years [1][2][3][4][5][6][7]. The PAT family is comprised of four members (PAT1-PAT4, SLC36A1-4); the PAT proteins consist of around 470-500 amino acids and are thought to represent integral membrane proteins with a > 60% similarity to each other [8].…”

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confidence: 99%

“…The proton/amino acid transporter family PAT (SLC36) has been identified from human, mouse and rat origin during the last three years [1][2][3][4][5][6][7]. The PAT family is comprised of four members (PAT1-PAT4, SLC36A1-4); the PAT proteins consist of around 470-500 amino acids and are thought to represent integral membrane proteins with a > 60% similarity to each other [8].…”

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confidence: 99%

“…PAT1 recognizes, besides L-a amino acids, a number of additional substrates, e.g. b-alanine, c-aminobutyrate (GABA), betaine, D-Ser, and D-Ala [1,2,5,6,9], whereas for the PAT2 transporter only sarcosine has been identified as an additional high affinity substrate beside the normal L-a amino acid substrates [2,10].Recent studies on PAT1 suggest it to play a dual role in mammalian cells [8]. Based on its localization in lysosomal membranes in neurons [1,6] it is considered to act as an export system for amino acids out of lysosomes after their intralysosomal release from proteolytic processes.…”

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Substrate specificity and transport mode of the proton‐dependent amino acid transporter mPAT2

Foltz

Oechsler

Boll

et al. 2004

European Journal of Biochemistry

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The PAT2 transporter has been shown to act as an electrogenic proton/amino acid symporter. The PAT2 cDNA has been cloned from various human, mouse and rat tissues and belongs to a group of four genes (pat1 to pat4) with PAT3 and PAT4 still resembling orphan transporters. The first immunolocalization studies demonstrated that the PAT2 protein is found in the murine central nervous system in neuronal cells with a proposed role in the intra and/or intercellular amino acid transport. Here we provide a detailed analysis of the transport mode and substrate specificity of the murine PAT2 transporter after expression in Xenopus laevis oocytes, by electrophysiological techniques and flux studies. The structural requirements to the PAT2 substrates -when considering both low and high affinity type substrates -are similar to those reported for the PAT1 protein with the essential features of a free carboxy group and a small side chain. For high affinity binding, however, PAT2 requires the amino group to be located in an a-position, tolerates only one methyl function attached to the amino group and is highly selective for the L-enantiomers. Electrophysiological analysis revealed pronounced effects of membrane potential on proton binding affinity, but substrate affinities and maximal transport currents only modestly respond to changes in membrane voltage. Whereas substrate affinity is dependent on extracellular pH, proton binding affinity to PAT2 is substrate-independent, favouring a sequential binding of proton followed by substrate. Maximal transport currents are substrate-dependent which suggests that the translocation of the loaded carrier to the internal side is the rate-limiting step.Keywords: electrophysiology; functional characterization; proton symporter; substrate recognition; transport mode.The proton/amino acid transporter family PAT (SLC36) has been identified from human, mouse and rat origin during the last three years [1][2][3][4][5][6][7]. The PAT family is comprised of four members (PAT1-PAT4, SLC36A1-4); the PAT proteins consist of around 470-500 amino acids and are thought to represent integral membrane proteins with a > 60% similarity to each other [8]. The orthologous proteins from mouse, rat and human show an identity of more than 90% to each other. The expression pattern of the four different transporter mRNAs is quite different. The PAT1 mRNA shows widespread expression with high levels in brain, intestine and kidney whereas the PAT2 mRNA is highly abundant in lung, kidney and brain. PAT3 mRNA is found solely in testis, whereas PAT4 mRNA shows ubiquitous expression [8].So far, only PAT1 and PAT2 have been characterized functionally. They have an exceptional position among the mammalian amino acid transporters, as they act as electrogenic amino acid/proton symporters. Transport is dependent on the extracellular pH, but is independent of sodium, chloride, and potassium ions [1,2,4,7]. Moreover, PAT1 and PAT2 mediated amino acid influx leads to a pronounced intracellular acidification [2,9] by cotransport ...

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confidence: 99%

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Substrate specificity and transport mode of the proton‐dependent amino acid transporter mPAT2

Foltz

Oechsler

Boll

et al. 2004

European Journal of Biochemistry

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Glycosylation affects the stability and subcellular distribution of human PAT1 protein

Luo

Zhao

et al. 2017

FEBS Letters

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The amino acid transporter PAT1 is typically expressed on the lysosome and plasma membranes in various human tissues. Glycosylation has been shown to be critical for the cell surface expression of PAT1, but not for its stability, in Xenopus oocytes. Here, we report that the glycosylation-deficient mutant of PAT1 (PAT1 ) is unstable and is degraded mainly via the endoplasmic reticulum-associated degradation pathway in HEK293 cells. Interestingly, PAT1 binds preferentially to the plasma membrane rather than to the lysosome. Consistent with this altered distribution, overexpression of PAT1 fails to inhibit the mechanistic target of rapamycin complex 1 (mTORC1). Our data suggest that glycosylation affects the stability and localization of PAT1 in HEK293 cells and the subcellular distribution of PAT1 is a factor affecting mTORC1 activity.

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Amino acids suppress the expression of PAT1 on lysosomes via inducing the cleavage of a targeting signal

Zhao

Luo

et al. 2017

FEBS Letters

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The lysosome-associated transporter proton-coupled amino acid transporter 1 (PAT1) promotes nutrient recycling through releasing luminal amino acids into the cytosol. Using HEK293 cells expressing an EGFP-tagged PAT1 (EGFP-PAT1) as a model, we identified a consensus tyrosine-based targeting signal in the cytosolic N-terminal region of PAT1, which facilitates its expression on the lysosome. Interestingly, this signal can be removed via protein cleavage in an amino acid-sensitive manner. The cleavage is suppressed upon amino acid starvation and is induced by amino acid replenishment. However, amino acid deficiency does not suppress the cleavage of amino acid-binding mutants of EGFP-PAT1. Our data support a mechanism, whereby amino acid binding induces PAT1 cleavage to remove a targeting signal, thus suppressing the expression of PAT1 on the lysosome.

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Functional Characterization of Two Novel Mammalian Electrogenic Proton-dependent Amino Acid Cotransporters

Cited by 154 publications

References 24 publications

Substrate specificity and transport mode of the proton‐dependent amino acid transporter mPAT2

Substrate specificity and transport mode of the proton‐dependent amino acid transporter mPAT2

Glycosylation affects the stability and subcellular distribution of human PAT1 protein

Amino acids suppress the expression of PAT1 on lysosomes via inducing the cleavage of a targeting signal

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