68
3.2 Basic UV-VIS-IR Absorption, Emission, and Elastic Light Scattering Methods
Saffman–Delbrück equations (see Saffman, 1975; Hughes, 1981). Here, the frictional drag γ
of a rotating cylinder is approximated as
(3.15)
ϒ =
+
(
)
( ) =
( )
4
8
1
2
π µ
µ
ε
πη
ε
rC
rC
c
We assume the viscosities of the watery environment just outside the cell membrane and just
inside the cell cytoplasm (μ1 and μ2, respectively) are approximately the same, ηc (typically
~0.001–0.003 Pa·s). The dimensionless parameter ε is given by
(3.16)
ε
µ
µ
η
η
η
= (
)
+
(
) =
r h
r
h
/
m
c
m
1
2
2
The viscosity of the phospholipid bilayer is given by the parameter ηm (~100–1000 times
greater than ηc depending on both the specific phospholipids present and the local molecular
architecture of nonlipids in the membrane). The parameter C can be approximated as
(3.17)
C
c
O
ε
ε
ε
ε π
ε
ε
ε
( )
−+
−
(
) +
(
)
−
ln / )
/
ln
/
(2
4
2
2
2
2
1
Here c is Euler–Mascheroni constant (approximately 0.5772). The effective rotational
diffusion coefficient can then be calculated in the usual way using the Stokes–Einstein rela
tion and then the rotational correlation time is estimated.
Typical nanometer length scale fluorophores in the watery cytoplasm of cells have rota
tional correlation times of a few nanoseconds (ns), compared to a few microseconds (μs) in a
typical phospholipid bilayer. These parameters can be measured directly using time-resolved
anisotropy, with a suitable fluorescence polarization spectrometer that can typically perform
sub-nanosecond sampling. The application of fluorescence anisotropy to cellular samples,
typically in a culture medium containing many thousands of cells, offers a powerful method
to probe the dynamics of protein complexes that, importantly, can be related back to the
actual structure of the complexes (see Piston, 2010), which has an advantage over standard
fluorescence microscopy methods.