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First published online October 31, 2008
Journal of Experimental Biology 211, 3594-3600 (2008)
Published by The Company of Biologists 2008
doi: 10.1242/jeb.021923
FRAP analysis of molecular diffusion inside sea-urchin spermatozoa
Department of Life Science, Graduate School of Arts and Sciences, The University of Tokyo, Komaba 3-8-1, Meguro, Tokyo 153-8902, Japan
* Author for correspondence at present address: Department of Biological Sciences, Faculty of Science and Engineering, Chuo University, Kasuga 1-13-27, Bunkyo-ku, Tokyo 112, Japan (e-mail: kam{at}myad.jp)
Accepted 18 September 2008
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Summary |
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 TOP Summary INTRODUCTIONMATERIALS AND METHODSRESULTSDISCUSSIONAPPENDIXReferences |
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Key words: FRAP, diffusion constants, intra-flagellar transport, molecular mobility
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INTRODUCTION |
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TOPSummaryINTRODUCTIONMATERIALS AND METHODSRESULTSDISCUSSIONAPPENDIXReferences |
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). So far, several reports have been presented
(Brokaw, 1966;
Nevo and Rikmenspoel, 1970;
Tombes et al., 1987) showing
theoretical simulations of energy transportation along beating flagella.
However, these studies used the diffusion coefficients of ATP or PCr, obtained
in aqueous solution (Brokaw,
1966; Nevo and Rikmenspoel,
1970) or in muscle fibers
(Tombes et al., 1987), because
no appropriate data acquired by the direct analysis of diffusion was
available. Since the cytoplasmic space inside the flagellum is largely
occupied by the structural components of axonemes
(Nicastro et al., 2005),
apparent molecular mobility under such crowded conditions might be severely
restricted compared with that in typical cell cytoplasm. Hence, direct studies
on diffusion rates have been expected to elucidate such detailed features.
Fluorescence recovery after photobleaching (FRAP) has been established as a
method to determine the diffusion coefficients in live cells
(Ladha et al., 1994;
Wey and Cone, 1981;
Yguerabide et al., 1982). In
FRAP, a small region of interest is photobleached by a laser pulse and
diffusion coefficients can be determined by measuring the time course of
fluorescence recovery. In the current work, we performed FRAP experiments to
determine the apparent diffusion coefficients of small fluorescent probes,
calcein, carboxyfluorescein and Oregon Green in both flagella and aqueous
solutions. These results provide the first direct determination of
intra-flagellar diffusion rates.
The second area of interest was diffusion and material transportation
between head and flagellum. During the activation of motility and the
preparation for fertilization, spermatozoa undergo a sequential change of the
concentrations of ions and signaling messengers that function as essential cue
chemicals affecting the flagellar motility and acrosomal reactions
(Darszon et al., 2001). It is
therefore likely that, for these ions and signals to work at an exact place
and time, they are compartmentalized in a specific region in spermatozoa. By
electron microscopy the `neck' region between head and flagellum was shown to
be densely packed in mammalian sperm
(Pessh and Bergmann, 2006). In
addition, the presence of diffusion barriers has been reported in the plasma
membrane of mammalian sperm (James et al.,
2004; Ladha et al.,
1997; Mackie et al.,
2001). Such evidence suggests that there could be an intracellular
diffusion barrier around the neck region. Although recent detailed information
on the active intra-flagellar transport (IFT) systems along cilia and flagella
revealed their critical roles in the structural and functional maintenance of
axonemes (Rosenbaum and Witman,
2002), another possible path of material diffusion beyond the neck
region has not been described. We analyzed fluorescence recovery in the head
region of sperm and investigated whether the molecular mobility through the
neck region is restricted.
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MATERIALS AND METHODS |
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TOPSummaryINTRODUCTIONMATERIALS AND METHODSRESULTSDISCUSSIONAPPENDIXReferences |
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Spawned sperm from sea urchin, Pseudocentrotus depressus A. Agassiz, were obtained by intracoelomic injection of 0.5 mol l–1 KCl. Collected sperm (dry sperm) were stored without dilution at 4°C until use. Artificial sea water (ASW) containing 460 mmol l–1 NaCl, 10 mmol l–1 KCl, 23 mmol l–1 MgCl2, 0.1 mmol l–1 EDTA, 10 mmol l–1 CaCl2 and 10 mmol l–1 MES (pH 6.0) or 10 mmol l–1 HEPES (pH 7.0) was used as the experimental medium.
Loading of fluorescent probes into sea-urchin spermatozoa
In order to load fluorescent probes into sea urchin spermatozoa, we used
the method previously described by Rodriguez and Darszon
(Rodriguez and Darszon, 2003)
with some modifications. Sperm were loaded with fluorescent probes by diluting
20 µl of dry sperm with 100µl of ASW (pH6.0) containing 20 µmol
l–1 AM or DA esters of fluorescent probes for 4 h at 4°C
in the dark. After the loading of probes, the remaining probes in the medium
were removed by centrifugation (2000 g, 3 min, 4°C). The
collected pellet of sperm was resuspended in 200 µl ASW (pH 6.0). The
washing procedure was repeated twice. The sperm pellet was finally suspended
in 100µl ASW (pH 6.0) and kept on ice until use.
Fluorescence recovery after photobleaching analysis
For the observation of conventional fluorescence images, an epifluorescence
microscope (IX-70; Olympus, Tokyo, Japan) with an Olympus U-MSWB filter-set
(for green fluorescence observations) was used. Specimens were observed under
the continuous illumination of a high-pressure mercury lamp. To avoid the
photobleaching of fluorescent probes, the mercury lamp light source was
attenuated with ND filters. Fluorescence images through an emission filter
were amplified with an image intensifier (C7787; Hamamatsu Photonics,
Hamamatsu, Japan) and collected on to a computer with a high speed CCD camera
system (HAS-200R; Ditect, Tokyo) at 200 f.p.s. Under these conditions, the
rate of photo-bleaching during image observation was low (
1/2
30 s) compared with the FRAP rates (2 s for full recovery) of dyes
we used.
For the photobleaching experiments of fluorescent probes, a 488 nm argon
laser (5500ASL; DZ Laser Service, Centerville, UT, USA) was used. The laser
beam was introduced into the microscope optics through an objective (UApo/340
x40/1.35 oil immersion lens; Olympus, Tokyo, Japan) by reflection using
a small rod mirror placed on the microscope optical axis just below the
objective. The intensity profile of the focused laser spot on the specimen
field was measured with the CCD camera and fitted to a Gaussian distribution,
which gave a spot radius parameter, 
, of 3.05 µm (1/e2).
The intensity and exposure time of bleaching laser pulses were modulated with
ND filters as well as a mechanical shutter (EC-598; Copal, Tokyo, Japan). The
mechanical shutter was controlled with a shutter driver (EN-609; Copal, Tokyo,
Japan) and a hand-made circuit using timer integrated circuits (LM555CN/NOPB;
National Semiconductor, Santa Clara, CA, USA). We also made the shutter
controller to switch off the image intensifier during photobleaching to avoid
damages by the high intensity illumination of the argon laser.
Spermatozoa that had been pre-loaded with fluorescent probes were diluted with ASW (pH 7.0) and placed in a chamber made of two coverslips separated with a pair of stripped plastic tape spacers. Spermatozoa were attached to the glass surfaces of coverslips and we used such spermatozoa for further observations. The specimen was then washed with 200 µl of ASW (pH 7.0) to remove remaining dye and free spermatozoa in the solution. To determine the diffusion coefficients in aqueous solutions by the FRAP experiments, 4 µl of experimental solutions containing 10 mmol l–1 HEPES (pH 7.0), 20–60% (v/v) glycerol, and 20 µmol l–1 fluorescent dye were placed between two coverslips without plastic tape spacers. In these cases, observed diffusion is two-dimensional. We used ImageJ (NIH, Bethesda, MD, USA) to determine the intensity of fluorescence in recorded images. All the FRAP experiments were carried out at room temperature (20–23°C).
For data analysis, we first obtained time constants, 1/2,
by fitting the time courses of fluorescence recovery in photobleached regions
to the following equation (Ladha et al.,
1994; Yguerabide et al.,
1982):
 | (1) |
are the fluorescence
intensities immediately after and at infinite time (>1 s) after the
photobleaching, respectively. 1/2 is the time required for the
half recovery of fluorescence. For fitting data to the theoretical equations
to obtain F0, F and
1/2, the least-square fitting algorithm programmed with
Mathematica (ver. 5.0, Wolfram Research, Champaign, IL, USA) was used.
Dx and Dxy, the diffusion coefficients
for one-dimensional and two-dimensional diffusions, respectively, are given by
the following expressions (Ladha et al.,
1994; Wey and Cone,
1981):
 | (2) |
 | (3) |
is the
half-width at 1/e2 intensity around the focusing point of the
photo-bleaching laser beam. β varies depending on the percentage of dye
photobleaching. We took β values ranging from 1.0–1.2 in our
experiments depending on the magnitude of bleaching (signal ratios before
vs after photobleaching) according to the theoretical estimation by
Yguerabide and colleagues (Yguerabide et
al., 1982).
Determination of head/flagellum volume ratio
By directing a photobleaching laser beam to the head region of spermatozoa,
we were also able to photobleach fluorescent dye in the heads. If the amount
of fluorescence recovery in the heads is equal to the loss in the flagellum,
and the total fluorescence of the whole spermatozoon is constant, we can
estimate the volume ratio of spaces fluorescent probes can access,
Vhead/Vflagellum, using the equation
expressed by:
 | (4) |
are the total
amounts of fluorescence in the flagellum immediately after and at infinite
time after photobleaching, respectively. Fh0 and
Fh are the same parameters for heads (see Appendix
for more details). |
RESULTS |
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TOPSummaryINTRODUCTIONMATERIALS AND METHODSRESULTSDISCUSSIONAPPENDIXReferences |
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6µm
in diameter corresponding to the focused region of laser beam in each recorded
image and measured the mean fluorescence brightness (ImageJ, ver. 1.3). Each
value normalized by the initial fluorescence intensity before photobleaching
was plotted against time as shown in Fig.
2. All the fluorescein-derivatives we used in the experiments
– calcein, carboxyfluorescein, and Oregon Green – showed similar
recovery rates (Fig.
2A–C), although their molecular masses are slightly
different. Their half-recovery times, 1/2, were around 100 ms,
which was slow enough for the time resolution of our image recording (5 ms).
Since the diameter of the flagellum is extremely small (0.2 µm)
compared with that of the bleached area (6 µm), it is reasonable to
consider the recovery curves of fluorescence as the results of simple
one-dimensional diffusion. Determined diffusion coefficients of these
fluorescence probes in flagella, Dfl, were 64, 64 and 63
µm2 s–1 for calcein (Mr,
622.54), carboxyfluorescein (Mr, 376.32) and Oregon Green
(Mr, 412.30), respectively
(Table 1).
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7 µm). A
small region in the thin aqueous layer was then photobleached by a laser pulse
in a similar way to the measurements using sperm flagella. In contrast to
flagella, the diffusion in this case should be regarded as occurring in two
dimensions (Kao et al., 1993;
Swaminathan et al., 1997).
Also, since the fluorescent probes diffuse faster than the time resolution of
our measuring system, we executed the experiment using various concentrations
of glycerol (viscosity, 1.76–10.8 mPa s) to reduce the diffusion rates.
Then, by extrapolating the results, we determined the diffusion coefficients
at 1 mPa s as in aqueous solution without glycerol. A typical example of a
fluorescence recovery curve in 20% glycerol solution (1.76 mPa s) is shown in
Fig. 2D.
Fig. 3 shows the relationship
between diffusion rates and the viscosity of the solvent for each probe. As
expected from the Einstein–Stokes equation, the reciprocal of the
diffusion coefficient, 1/D, varied proportionally with the viscosity
of the medium. Diffusion coefficients for the probes in aqueous solution
(viscosity, 1 mPa s), Daq, were determined by
extrapolating these data. As the measured diffusion coefficients tended to
scatter at higher viscosities for unknown reasons, data at 10.8 mPa s were
neglected for the least squares fitting, where we could assume the data were
with uniform variances according to the White test (P<0.01)
(White, 1980).
Daq was thus determined to be 337, 296 and 255
µm2 s–1 for calcein, carboxyfluorescein and
Oregon Green, respectively (see Table
1).
The ratios of diffusion coefficients determined in flagella to those determined in solution, Dfl/Daq, are also shown in Table 1. Diffusion coefficients we obtained were all lower in flagella compared to those in solution. The extent of the rate reductions varied slightly (0.19–0.25) depending on the species of probes.
Simulation of intraflagellar ATP diffusion
Simply assuming that the diffusion coefficient of ATP is similar to that of
fluorescein derivatives of similar molecular masses (60 µm2
s–1), the rate of ATP diffusion inside flagella is about
three times lower than that expected in previous calculations (D
150 µm2 s–1) by Tombes et al.
(Tombes et al., 1987). In
their model, ATP molecules are produced at the mitochondrion located at the
proximal end of the flagellum and provided by diffusion, together with the ADP
recycling system by creatine shuttle
(Tombes and Shapiro, 1985).
Using the same model, we simulated whether the energy could be sufficiently
provided along the flagellum (length, 40 µm) when the parameter of the
diffusion coefficient for ATP was set to 60 µm2
s–1 and the diffusion coefficients for other important
molecules were set as shown in Table
2 and Fig. 4. We
also calculated intraflagellar concentration profiles of ATP, ADP, AMP,
creatine (Cr) and PCr. Effects of competitive inhibition of dynein ATPase
activity by ADP as well as rate limiting effects of ADP recycling by the
creatine shuttle were included. We could repeat the results that ATP
concentration and dynein ATPase activity were high throughout the flagellum if
the ATP diffusion coefficient of 150 µm2 s–1
was used, however, both gradually decreased at the tip of the flagellum when
we used the diffusion coefficient of 60 µm2 s–1
(Fig. 4A,C). If we executed the
same simulation in sperm flagella of 100 µm of length, we found energy
supply was not enough at either rates of diffusion (60 or 150
µm2 s–1;
Fig. 4B,D). In such a long
flagellum, even if the ADP recycling system by the creatine shuttle is
working, dynein ATPase activity is assumed to be significantly decreased at
the distal portion of the flagellum at both diffusion rates, retarding
flagellar beating as in the case of normal flagellar length (40µm) with
reduced creatine kinase activity (Tombes
et al., 1987).
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Diffusion between the head and flagellum
To investigate whether small probe molecules can go through the proximal
basal-body region into the head, we directed a photobleaching pulse on the
whole head region of a calcein-loaded spermatozoon. After bleaching, we
observed gradual recovery of head fluorescence along with concomitant decrease
in flagellar fluorescence signals (Fig.
2E). The half-recovery time, 1/2, was
6.8±1.5 s (N=5), which was more than 60 times longer comparing
with that of intraflagellar FRAP. Since there was no detectable change in the
total amount of calcein molecules in the whole spermatozoon during the
recovery, it is likely that we observed the slow diffusion of fluorescent
probes from flagella to heads. Using Eqn
4 (see the Appendix as well), we determined the head/flagellum
volume ratio of spaces where calcein can diffuse. The determined volume ratio,
Vhead/Vflagellum was 4.6±1.9
(N=5).
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DISCUSSION |
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150 to 500 µm2 s–1
(Brown et al., 1999;
Culbertson et al., 2002;
Mustafa et al., 1993;
Politz et al., 1998). Such a
large variation was most probably the result of the differences in measuring
methods or conditions rather than the differences in probe properties (e.g.
molecular mass, shapes or charges). The Daq values we
obtained in this study were 337, 296 and 255 µm2
s–1 for calcein, carboxyfluorescein and Oregon Green,
respectively (Table 1). All of
these Daq values were comparable to those previously
reported, thus, confirming the accuracy of FRAP analysis by our system.
The ratios, Dfl/Daq, were 0.19,
0.22 and 0.25 for calcein, carboxyfluorescein and Oregon Green, respectively
(Table 1). One of the possible
explanations for these 80% reductions of Dfl relative
to Daq is that electrostatic interactions with the crowded
components of axoneme attenuated the apparent Dfl. Another
possibility, that these probes might be attached to intra-flagellar
macromolecules that diffuse slowly, could not be fully excluded under our
experimental conditions, so the values we obtained could reflect apparent
diffusion rates affected by such macromolecules, if any, as well as by
intra-flagellar viscosity and crowded effects. Our observation suggests that
molecular mobility inside sperm cells would not simply depend on diffusion by
random walk but on some interactions with intra-flagellar components, although
whether it is specific or non-specific is unclear at present. Alternatively,
the reduction of Dfl may be due to the restricted aqueous
volume in the flagella where the cross section is mostly filled with axonemal
structures. In mammalian nerve cells, diffusion coefficients of the
Ca2+-binding protein parvalbumin and fluorescein-labeled dextran
have been reported to be 10 µm2 s–1 in
both axonal and somatic cytoplasm, but 40 µm2
s–1 in dendrites (Schmidt
et al., 2007), suggesting that, instead of cell shapes, molecular
interaction with intracellular components would be the major factor reducing
intracellular diffusional mobility. This could also be the case in sperm
flagella. Further detailed investigations are required to determine the major
factors in the reduction of diffusion coefficients in flagella.
In the case of sea-urchin sperm flagella, the only energy source for
flagellar motility is mitochondria located near the proximal ends. It has been
described that an additional energy transferring system known as the `creatine
shuttle' is also present in sea urchin sperm
(Tombes and Shapiro, 1985). By
simulating the rates of ATP consumption and supply by diffusion of ATP and
PCr, Tombes et al. (Tombes et al.,
1987) concluded that enough ATP could only be provided from
mitochondria to a flagellar tip when the creatine shuttle system is working.
However, in their calculations, they used a diffusion coefficient for ATP of
150 µm2 s–1, which was indirectly obtained from
the recovery rates of contraction force in muscle fibers
(Bowen and Martin, 1963), as no
appropriate data for diffusion coefficients in flagella was available. In the
current work, we determined Dfl for three fluorescent
probes to be 60 µm2 s–1 which is about one
third of that in muscle fibers (>150 µm2
s–1). Here, we again similarly calculated ATP diffusion by
assuming Dfl of ATP and PCr to be 60 and 104
µm2 s–1, respectively
(Table 2). It was revealed that
ATP concentration gradually decreases toward the tip
(Fig. 4A). However, even at the
tip (40 µm from the proximal end of flagellum), ATP concentration was still
maintained at more than 2 mmol l–1 if the ATP concentration
at the proximal end was as high as 6 mmol l–1 and if the
creatine shuttle system is working. This ATP concentration, even at the distal
ends, would be high enough for the full activation of flagellar ATPases and
bending motions, which have a Km of about 100 µmol
l–1 (Gibbons and Gibbons,
1972). Even if there was competitive inhibition of dynein ATPase
activity by accumulated ADP (Okuno and
Brokaw, 1979), ATPase activity should still be kept high enough to
sustain flagellar beating (Fig.
4C). Therefore, even if diffusion rates are three times smaller
than those in muscle fibers, sea urchin sperm flagella with a creatine shuttle
system could maintain continuous beating.
Using the same diffusion parameters, we also calculated the length limit of
flagella (Fig. 4B,D). In the
case with a flagellum longer than 60 µm, the tip concentration of ATP was
estimated to be lower than 100 µmol l–1
(Fig. 4B,D), a problematic
concentration to maintain regular beating. Even if the diffusion coefficients
of ATP and PCr are 150 and 260 µm2 s–1,
respectively (Table 2), the
maximum possible length of a flagellum is 100 µm in this model
(Fig. 4B). Dynein ATPase
activities seem to be significantly decreased in both cases
(Fig. 4B,D). In many other
cases, the flagella of mammalian spermatozoa are longer than this (e.g.
150 µm for mouse spermatozoa) and our calculation indicates that a
simple diffusion pathway by itself cannot provide full energy for flagellar
movements. Indeed, unlike sea urchin spermatozoa, it has been reported that
mammalian sperm have glycolytic enzymes in the tail region and this metabolic
pathway may play the major role in providing ATP
(Mukai and Okuno, 2004).
Without such a system providing ATP, flagella longer than 60 µm, as in the
case of other invertebrate spermatozoa and dinoflagellates, for example, could
solve the problem by other means. For example, making flagellar diameter
larger so as to produce larger diffusion channels, reducing intarcellular
obstacles to ATP mobility, or beating with lower frequency and smaller bend
amplitudes in order to save ATP consumption could be possible options. An
active ATP/PCr transport system along flagella might be a possible solution,
although we have no evidence so far.
We were also interested in the material diffusion through the neck region
since specific structures in the basal body region, including membrane
necklace-like structures, could be working as diffusion barriers. Electron
microscopy analyses have shown that the proximal ends of flagella of mammalian
spermatozoa (Pessh and Bergmann,
2006) and an alga, Chlamydomonas reinhardtii
(Mitchell et al., 2005), are
densely packed, which may restrict the diffusivity and would be possible
candidates as diffusion barriers between flagella and heads (or cell bodies).
These structural obstacles may function generally as diffusion barriers in
other types of eukaryotic cilia and flagella. Therefore, the active
intra-flagellar transport (IFT) must be a vital system in forming the
structure and maintaining the functions of cilia and flagella in many cases
(Bisgrove and Yost, 2006;
Rosenbaum and Witman, 2002).
In similar FRAP experiments with calcein, we observed fluorescence recovery in
the head region (Fig. 2E). We
found head fluorescence recovery, with a half-recovery time
(1/2) of 6.8±1.5 s (N=5), indicating calcein
could move between head and flagellar regions. Note that in flagella,
1/2 was around 100 ms; thus, the fluorescence recovery rate
was more than 60 times slower in the head than in the flagellum. Unlike the
cylindrical shape of flagellum, the head spreads three-dimensionally and it is
difficult to simply compare the FRAP rates between the head and flagellum.
However, the apparent diffusion rate at the neck region was obviously lower
than that in the tail region, suggesting the presence of a diffusion barrier
around the neck region of spermatozoa. It is currently not clear whether the
barrier is on the head side or flagellar side of the mitochondrion, or whether
the mitochondrion itself would be a structural barrier for diffusion. If
diffusion is restricted between mitochondrial and tail regions, some
mechanism, such as a molecular filter, should exist to move molecules such as
ATP or PCr from the mitochondrion to the flagellum, although this requires
further investigation. How the diffusion barrier between head and flagellum,
if present, can be generalized to other cells and how the IFT system is
compromising or co-operating with the diffusion hurdles remain to be
clarified.
From the data obtained from the FRAP experiments of heads, we next estimated Vhead/Vflagellum, the ratio of head/flagellum volume of the space that calcein molecules can access. The obtained value of Vhead/Vflagellum was 4.6±1.9, corresponding to 82% of the volume of the head and 18% of the flagellum. If we assume that a sperm head is a sphere with a diameter of 3.8 µm and the flagellum is a cylinder of 0.2 µm diameter and 40 µm length, then Vhead/Vflagellum is estimated to be 23. Thus, the morphologically estimated volume percentages are 96% for head and 4% for flagellum. The value we obtained is reasonable because the structural components inside heads, such as DNA and acrosomes that are essential for fertilization and reproductions, are expected to be packed tightly, that is, heads are not simple, empty spheres.
In our current work, apparent diffusion coefficients for fluorescein-derived probes in flagella were determined and it was confirmed that calcein molecules can diffuse between the head and the flagellum. Our FRAP experimental system can, in principle, be applied to determine the diffusion coefficients even in motile flagella. Along with the analysis of the diffusion of macromolecules such as dextran-conjugated dyes or GFP, we expect that we will be able to clarify more detailed features of molecular diffusion and, thus, energy and material transportation in flagella as well as the biological significance of intra-spermatozoa compartmentalization.
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APPENDIX |
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TOPSummaryINTRODUCTIONMATERIALS AND METHODSRESULTSDISCUSSIONAPPENDIXReferences |
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1/2 7 s)
was observed as well as the concomitant decrease of fluorescence in the tail
region. Such observations led us to estimate the ratio of head/flagellum
volume as follows.
When the sperm head was photobleached, the total amount of fluorescent
probe in the tail region, Sf0 (at t=0), is given
by:
 | (A1) |
 | (A2) |
After fluorescence in the head area is finally recovered (at
t=), the total amounts of fluorescence probe in the flagellum
(Sf) and in the head
(Sh) are expressed by:
 | (A3) |
 | (A4) |
, Ch,
Ca and Cm are the final
concentrations of fluorescent probes (at t=) in the flagellum,
head, acrosome and mitochondrion, respectively. If all the fluorescence
recovery in the head region is by probe diffusion from the flagellum:
 | (A5) |
 |
 | (A6) |
and Ch are equal
at t=, Eqn A6
can be transformed into:
 | (A7) |
 | (A8) |
 | (A9) |
are the
observed intensities of total fluorescence in the flagellum at t=0
and t=, respectively, and Fh0 and
Fh are those in the head. Thus, from Eqns
A7,
A8,
A9, the volume ratio is
determined by the following equation:
 |
This final equation is the same as Eqn 4 in Materials and methods.
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Acknowledgments |
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References |
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TOPSummaryINTRODUCTIONMATERIALS AND METHODSRESULTSDISCUSSIONAPPENDIXReferences |
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