Mapping the alpha-subunit site photolabeled by the noncompetitive inhibitor [3H]quinacrine azide in the active state of the nicotinic acetylcholine receptor

We have characterized the time-resolved labeling of a site on the Torpedo californica electrocyte acetylcholine receptor (ACHR) by the photoreactive noncompetitive inhibitor derivative quinacrine azide (QA). The dependence of [3H]QA labeling on acetylcholine (ACH) concentration and on time is consis...

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Bibliographic Details
Published in:The Journal of biological chemistry 1990-07, Vol.265 (19), p.11017-11029
Main Authors: DIPAOLA, M, KAO, P. N, KARLIN, A
Format: Article
Language:English
Subjects:
Acetylcholine - metabolism
Affinity Labels
Amino Acid Sequence
Amphibian Venoms - pharmacology
Animals
Azides - metabolism
Binding Sites
Biological and medical sciences
Bupivacaine - pharmacology
Cell receptors
Cell structures and functions
Chlorpromazine - pharmacology
Chromatography, High Pressure Liquid
Cyanogen Bromide
Fundamental and applied biological sciences. Psychology
Molecular and cellular biology
Molecular Sequence Data
Molecular Weight
Monoamines receptors (catecholamine, serotonine, histamine, acetylcholine)
Nicotinic Antagonists
Peptide Fragments - isolation & purification
Peptide Mapping
Photochemistry
Proadifen - pharmacology
Quinacrine - pharmacology
Receptors, Nicotinic - metabolism
Torpedo
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Summary:We have characterized the time-resolved labeling of a site on the Torpedo californica electrocyte acetylcholine receptor (ACHR) by the photoreactive noncompetitive inhibitor derivative quinacrine azide (QA). The dependence of [3H]QA labeling on acetylcholine (ACH) concentration and on time is consistent with the preferential labeling by [3H]QA of ACHR in the open state. The ACH-dependent [3H]QA labeling, which was associated predominantly with the alpha-subunit, was blocked by other noncompetitive inhibitors including quinacrine, chlorpromazine, proadifen, histrionicotoxin, and bupivacaine. alpha-Subunit from ACHR labeled with [3H]QA 20 ms after the addition of ACH was cleaved with CNBr, and the fragments were separated by high pressure liquid chromatography. A peptide containing a major site of specific labeling was purified on two different reverse-phase columns. By N-terminal sequencing, amino acid composition, binding to mercurial-agarose, and apparent molecular weight, this [3H]QA-labeled peptide was identified as alpha-208-243, a CNBr fragment containing the putative membrane-spanning helix M1.
ISSN:0021-9258
1083-351X
DOI:10.1016/S0021-9258(19)38551-5