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Volume 271,
Number 6,
Issue of February 9, 1996 pp. 3085-3090
©1996 by The American Society for Biochemistry and Molecular Biology, Inc.
Lateral
Organization of Pyrene-labeled Lipids in Bilayers as Determined from
the Deviation from Equilibrium between Pyrene Monomers and Excimers
(Received for publication, September 21, 1995; and in revised form, November 14, 1995)
Yechezkel
Barenholz
, ,
Tina
Cohen
,
Elisha
Haas
,
Michael
Ottolenghi
In lipid bilayers, pyrene and pyrene-labeled lipids form
excimers in a concentration-dependent manner. The aromatic amine N,N-diethylaniline (DEA), which has a high
membrane-to-medium partition coefficient, quenches the monomers only,
and therefore it is expected that under conditions in which the
monomers are in equilibrium with the excimers due to the mass law, the
Stern-Volmer coefficient (K ) for monomers (M),
defined as K , should be identical to that of the
excimer (E), defined as K , and K /K = 1.0. This is
indeed the case for pyrene and pyrene valerate in egg
phosphatidylcholine small unilamellar vesicles. However, for pyrene
decanoate and pyrene dodecanoate in these vesicles, and for N-[12-(1-pyrenyl)dodecanoyl]sphingosylphosphocholine
in a matrix of either N-stearoyl sphingosylphosphocholine or
1-palmitoyl-2-oleoyl phosphatidylcholine, K < K . This can be explained either by the existence
of (a) two subpopulations of excimers, one in fast equilibrium
with the monomers and the other, related to ground-state
protoaggregates of pyrene lipids; (b) two monomer
subpopulations where part of M cannot be quenched by DEA; or (c) two monomer subpopulations, both quenched by DEA, but only
one of which produces excimers. The good agreement between the
photophysical processes determined by steady state and time-resolved
measurements supports the third explanation for the bilayers containing
pyrene phospholipids. It also suggests that the main factors
determining the immiscibility of pyrene lipids in phospholipid bilayers
are the temperature, the difference in the gel-to-liquid-crystalline
phase transition temperature ( T )
between the matrix and the pyrene lipid, and the structural differences
between the matrix lipid and the pyrene-labeled lipid. These results
indicate that the K /K ratio
can serve as a very sensitive tool to quantify isothermal microscopic
immiscibility in membranes. This novel approach has the following
advantages: applicability to fluid phase immiscibility, requirement of
a relatively low mol fraction of pyrene lipids, and conceivably,
applicability to biological membranes.

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Copyright © 1996 by the American Society for Biochemistry and Molecular Biology.
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