Acutely altered hemodynamics following venous obstruction in the early chick embryo
1 Department of Obstetrics and Gynaecology, Erasmus MC, Rotterdam, The
Netherlands
2 Department of Epidemiology and Biostatistics, Erasmus MC, Rotterdam, The
Netherlands
3 Department of Anatomy and Embryology, Leiden University Medical Center,
Leiden, The Netherlands
* Author for correspondence (e-mail: n.ursem{at}erasmusmc.nl)
Accepted 10 January 2003
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Summary |
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Key words: chick embryo, Doppler ultrasound, hemodynamics, blood flow velocity, venous clip model
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Introduction |
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The chick embryo has been used as a model for many decades because in many
aspects the embryonic chick heart resembles the developing human heart
(Clark and Hu, 1982;
Nakazawa et al., 1988
). An
intervention model for the chick embryo was designed to obtain insight into
the long-term hemodynamic effects of altered venous return patterns on cardiac
morphogenesis and malformations. Specific cardiac malformations were induced
by permanently obstructing the right lateral vitelline vein with a microclip
(venous clip model; Hogers et al.,
1997
), thereby altering the intracardiac blood flow patterns. A
spectrum of outflow tract anomalies can be induced by this intervention.
Hogers et al. (1997
)
postulated that alterations in hemodynamic parameters could lead to changes in
shear stress, which could alter the expression of shear-stress-responsive
genes with downstream alterations in developmental processes, resulting in
cardiac malformations. The observation of intracardiac blood flow pattern
alterations during clipping, visualised by injected India ink, suggested that
hemodynamics is influenced by clipping
(Hogers et al., 1999
). Other
studies have also shown that alterations in hemodynamics can precede the onset
of structural defects (Stewart et al.,
1986
).
A previous study from our group demonstrated that at stage 34 (day 8 of
incubation) heart rate was decreased in embryos that had been clipped at stage
17 (stages according to Hamburger and
Hamilton, 1951), whereas peak systolic and mean systolic
velocities, as well as peak and mean blood flow, were increased compared to
normal embryos (Broekhuizen et al.,
1999
). These results showed the presence of long-term hemodynamic
changes after clipping. However, at this point (stage 34) cardiac
malformations are already present, so it is impossible to discriminate between
the effects of cardiac malformations and any direct effects of clipping on
hemodynamics.
By a modification of the method used for Doppler frequency detection it is
now possible to obtain good quality waveforms directly after clipping at stage
17 (Ursem et al., 2001). This
allows examination of the direct effects of clipping on hemodynamics, to
improve our understanding of how cardiac anomalies may arise following venous
obstruction. We hypothesise that cardiac malformations induced by clipping are
caused by instantaneous changes in blood flow through the heart resulting in
altered activation of shear-stress-responsive genes. In the present work we
show the instantaneous effects of clipping the right lateral vitelline vein on
hemodynamics in the stage 17 (52-64 h of incubation) chick embryo.
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Materials and methods |
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Measurements
Eight dorsal aortic blood flow velocity measurements were made per embryo.
The first velocity measurement (baseline) was done directly after exposure of
the embryo. The second measurement was performed directly after successful
clipping of the right vitelline vein at approximately 4 min from the first
measurement. For each clipped embryo a control embryo was measured, matched
for the exact time interval between the first measurement before clipping and
the second measurement directly after clipping. This was important since
cooling of the embryo would take place despite the use of a thermoelement, and
cooling influences the outcome of the measurements
(Nakazawa et al., 1985;
Wispé et al., 1983
).
The third measurement was performed 30 min after clipping, and the fourth to
eighth recordings at 1, 2, 3, 4 and 5 h after clipping, respectively. The
control embryos were subjected to the same measurement schedule as
venous-clipped embryos.
Materials
Dorsal aortic blood flow velocity was measured using a 20 MHz pulsed
Doppler meter (model 545C-4, Iowa Doppler Products, Iowa City, IA, USA). The
Doppler audio signals were digitised at 12 kHz and stored on hard disk. Using
complex fast Fourier transform analysis, the maximum velocity waveform was
reconstructed. A more detailed description of this method has been published
previously (Ursem et al.,
2001). The Doppler probe, consisting of a 750 µm piezoelectric
crystal, was positioned at an angle of 45° to the dorsal aorta at the
level of the developing wing bud. The sample volume was adjusted to cover the
lumen of the dorsal aorta only, excluding other adjacent vessels. The internal
aortic diameter was measured at the same level by video imaging using a stereo
microscope (model SV 6, Carl Zeiss, Oberkochen, Germany) and a video camera
(model SSC-M370CE, Sony Corporation, Tokyo, Japan). The video images were
acquired with an image acquisition board (IMAQ PCI-1408, National Instruments,
Austin, TX, USA) and subsequently analysed using a custom-built analysis
program using IMAQ Vision software (National Instruments). Size calibration in
the horizontal and vertical planes of the image was performed by videotaping a
scale divided into 10 µm divisions. Aortic diameter was calculated by
incorporating the magnified video image displaying the dorsal aorta into the
image analysis program.
Blood flow Q was calculated from
Q=d2/4, where
is mean aortic blood flow velocity
and d is the internal aortic diameter. Peak acceleration
(d
/dt) was derived from the
dorsal aortic blood flow velocity by means of digital differentiation. Stroke
volume was determined from the quotient of the dorsal aortic blood flow and
the heart rate. We determined peak systolic velocity (PSV, mm s-1),
time-averaged velocity (TAV, mm s-1), heart rate (beats
min-1), peak blood flow (mm3 s-1), mean blood
flow (mm3 s-1), peak acceleration (mm s-2)
and stroke volume (mm3) for each cardiac cycle. For each embryo a
high quality waveform recording of 10 s was used for the analysis. The 10 s
recordings contain 20-27 heartbeats. For all hemodynamic parameters in each
embryo, the mean of all cardiac cycles was calculated.
Statistical analysis
Reproducibility study
The method by which we obtained the velocity waveform recordings of the
dorsal aorta in chick embryos using a 20 MHz pulsed Doppler meter, was
validated by conducting a separate study to assess its reproducibility. We
measured 10 embryos at HH 17 that showed no bleeding or deformities. All
experiments were performed in ovo. For each of the 10 embryos, 3
independent measurements were performed at 30 s time intervals. All the
measurements were performed by one investigator (S.S.) in the same order: the
egg was placed on the thermoelement under the dissecting microscope, the
Doppler probe was positioned and the recording was made. In between the
measurements the egg was removed from its position. The exact time interval
between the measurements was documented. The mean coefficient of variation
(CV, %) for heart rate, peak systolic velocity and time-averaged velocity was
calculated to determine intraobserver reproducibility. In the calculations,
the CV was adjusted for the trend due to cooling over the time points by
performing an analysis of variance (ANOVA). A common linear trend was assumed
for each embryo in this analysis. The resulting standard deviation (S.D.) of
residuals was taken as the S.D. of measurement error. All calculations and
statistical analyses were performed using SPSS 10.1 software (SPSS Inc,
Chicago, IL, USA).
Hemodynamics
Heart rate, PSV, TAV, peak blood flow, mean blood flow, peak acceleration
and stroke volume data are presented as mean ± standard error of the
mean (S.E.M.). Hemodynamic parameters were compared within and between groups.
Paired t-tests were performed within each group to compare mean
values at all time points with baseline values. Repeated measurements ANOVA,
using SAS PROC MIXED, was performed on the net changes from baseline level to
assess whether the profiles of the net changes paralleled each other. The
values were standardised by taking the net changes from baseline level in
order to adjust for biological variability. Net change profiles in a parallel
position indicated a significant difference in the net changes throughout the
5 h study period between the clipped and control groups. If the profiles
differed significantly from parallelism, paired t-tests were
performed at each time point to compare both groups. P<0.05 was
considered statistically significant.
Statistical analyses were performed using SPSS 10.1 and SAS 6.12 software (SAS Institute Inc, Cary, NC, USA).
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Results |
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Hemodynamics
The values (means ± S.E.M.) for all the measured parameters in the
clipped embryos (N=16) and control embryos (N=16) at all
time points are presented in Table
1. The baseline values of all parameters did not significantly
differ between both groups. The mean time required to place the microclip was
4 min (range 3.23-4.15 min), and the control group was matched for this 4 min
period to differentiate between the influence of cooling of the embryo and
clipping. All hemodynamic parameters decreased markedly during the venous clip
procedure in the clip group and the 4 min period in the control group.
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The profiles of changes from baseline level of all the parameters did not significantly differ from parallelism (P>0.05), except for heart rate and peak acceleration (P<0.05).
Directly after clipping or the 4 min period (controls), heart rate decreased significantly in both groups (Fig. 2A). This decrease was not significantly different between the groups. However, at 30 min, 1 h and 2 h the difference in heart rate between the clip and control group was significant. In the clipped group it took 3 h for the heart rate to gradually return to baseline level, whereas the control group showed a recovery within 30 min.
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The profile of the net changes in the PSV of the clipped group (Fig. 2B) was significantly below the profile of the control group (P<0.001). The clipped group demonstrated a 57% decrease in PSV after clipping as compared with a 19% decrease in the control group. This decrease stabilised at 30 min after clipping at ±22%. In the control group PSV was significantly elevated at all time points beyond 2 h compared to baseline level.
The profile of the net changes in TAV of the clipped group (Fig. 2C) was significantly lower than the profile of the control group (P<0.001). Following an initially significant decrease of 53% in the clipped group, TAV slowly stabilised at a level of 17% below baseline level. The control group recovered within 30 min and showed a significantly raised TAV at 4 and 5 h.
The profile of the net changes in peak blood flow of the clipped group (Fig. 2D) was significantly below the profile of the control group (P<0.001). Peak blood flow decreased by 58% directly after clipping as compared with 18% in the control group. This decrease in the clipped group stabilised significantly below the baseline level at 30 min after clipping. The control group displayed a significantly elevated peak blood flow after 3 h.
The profile of the net changes in mean blood flow of the clipped group (Fig. 2E) was significantly below the profile of the control group (P<0.001). In the clipped group mean blood flow was significantly lower directly after clipping, at 30 min and at 1 h after clipping as compared with baseline level. No significant differences existed at later time points. The control group only showed a significant decrease after the 4 min period and even demonstrated a significantly elevated level of mean blood flow at 4 and 5 h.
The profiles of net changes in peak acceleration (Fig. 2F) significantly (P<0.05) deviated from paralellism. The net changes in peak acceleration of the clipped group and the control group were significantly different at all time points. Within the clipped group peak acceleration was significantly decreased at all time points after clipping as compared with baseline level. The control group showed a significant decrease after the 4 min period only and a significant increase at all time points thereafter.
The profile of the net changes in stroke volume of the clipped group (Fig. 2G) was significantly lower than the profile of the control group (P<0.001). Stroke volume was significantly lower up to 1 h after clipping. At 4 and 5 h stroke volume was also significantly reduced. The control group demonstrated a significant decrease only immediately after the 4 min period.
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Discussion |
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A significant reduction after clipping is demonstrated for all hemodynamic
parameters, with a recovery seen for only 3 out of 7 parameters (heart rate,
time-averaged velocity and mean blood flow) during the 5 h study period. In
the control group all parameters recovered to baseline values and displayed an
additional increase after 5 h, as could be expected in a normally developing
embryo. It is likely that most if not all hemodynamic parameters in the
clipped group would recover within the next stages of development, especially
since Broekhuizen et al. (1999)
observed no significant differences in hemodynamic parameters at stage 24
between clipped and control embryos, except for a lower peak acceleration.
In the clipped group it was evident that the magnitude of decrease of the
hemodynamic parameters observed at the first measurement after clipping was
mainly due to the clipping, with additional effects due to cooling. In the
control group the observed hemodynamic changes after the 4 min period were due
to minor handling and to cooling of the embryo. It is known that chick embryo
hemodynamics is greatly influenced by temperature (Nakazawa et al.,
1985,
1986
;
Wispé et al., 1983
).
Prolonged incubation at low temperatures can even give rise to cardiac
malformations (de la Cruz et al.,
1966
). de la Cruz et al.
(1966
) observed cardiac
malformations in 18.8% of the embryos that had survived during continuous
incubation at 35.8°C until hatching. In the clip study by Hogers et al.
(1997
) the clipped embryos
were only subjected to cooling for approximately 4 min, as were our embryos.
In their study, specific cardiac malformations were induced in 64% of the
clipped embryos, which is much higher than the 18.8% cardiac malformations
observed by de la Cruz et al.
(1966
) during continuous
incubation at a low temperature. This supports the conclusion of Hogers et al.
(1997
) that the cardiac
malformations observed by them are caused by obstruction of the right lateral
vitelline vein.
When considering the first 30 min of the study period the clipped group was characterised by a significant drop in all hemodynamic parameters whereas in the control group there was a return to baseline level at 30 min. The clipped group also displayed a significantly larger decrease in each hemodynamic parameter as compared with the control group. The changes in the hemodynamic parameters during the first 30 min may be explained as follows. Blood, circulating in the segment of the yolk sac vascular bed that is normally drained by the right lateral vitelline vein, is blocked due to clipping and can therefore not return directly to the heart. Blood is captured in the vitelline vascular bed while the heart keeps on pumping blood into all segments of the vascular bed. Therefore, the actively circulating blood volume is decreased, which results in a drop in venous return or preload and subsequently cardiac stroke volume. The decrease in preload also results in a decrease in peak acceleration, reflecting cardiac contraction force.
During the remainder of the study period, observations in the clipped group
showed a full recovery for time-averaged velocity and mean blood flow 5 h
after clipping. All other parameters demonstrated a partial recovery that,
however, remained significantly below baseline level. From these observations
it can be assumed that the embryo compensates to maintain a steady blood
supply to all organs. With the development of the vitelline vascular bed,
vascular resistance and impedance decreases
(Hu and Clark, 1989;
Wagman et al., 1990
;
Yoshigi et al., 1997
). We
therefore postulate that when a part of the vitelline vascular bed is closed
off from the rest of the vascular bed, the vascular resistance will rise. Even
when the anastomosis is formed that permanently provides a detour of blood
flow towards the heart, the venous vascular resistance will remain elevated
because blood has to pass along a longer route to reach the heart. There is a
new steady state in the hemodynamic situation that at least meets the demands
of the embryo that are necessary to survive 5 h after clipping. When comparing
the clipped and control group, all hemodynamic parameters of the latter are
situated well above the baseline, except for stroke volume. These findings
probably reflect embryonic growth during the study period. As has been
described by others, hemodynamic parameters increase with growth of the embryo
(Broekhuizen et al., 1993
;
Hu and Clark, 1989
).
The effects of venous clip on heart rate are more complex. There is an
initial drop in heart rate in both the clipped and control groups at 4 min
which, however, is not significantly different between the groups. This
suggests a cooling effect rather than a clipping effect. As outlined above,
clipping causes an acute decrease in preload. It is known that heart rate does
not respond to acute alterations in loading conditions
(Keller et al., 1994).
However, at 30 min to 2 h after clipping heart rate remained significantly
lower than in control embryos. This suggests a direct influence on the
pacemaker function of the heart that prevents a quick and normal heart rate
recovery. The cardiac autonomic nervous system is not functional until HH 41,
which rules out any impact of this system on heart rate
(Higgins and Pappano, 1981
;
Pappano, 1977
). Nevertheless,
there is evidence of the presence of ß-adrenergic receptors in the
myocardium at day 2-2.5 of incubation and circulating neurohumoral agents
(Lipshultz et al., 1981
). The
sudden and persistent decrease in preload following clipping may trigger a
release of neurohumoral agents or a change in sensitivity for these agents,
resulting in a temporary decrease in heart rate.
The question arises as to how these hemodynamic changes relate to the
development of cardiac malformations. During normal cardiac development,
cardiac performance increases (Clark and
Hu, 1982; Clark et al.,
1986
) and results in gradual changes in shear stress that either
up- or downregulate the expression of shear-stress-responsive genes
(Malek et al., 1999
;
Topper and Gimbrone, 1999
).
In vitro studies have demonstrated that endothelial cells are
subjected to fluid shear stress as a result of blood flow and are aligned in
the direction of the flow (Malek and
Izumo, 1996
; Malek et al.,
1999
) and that changes in shear stress especially cause
alterations in gene expression (Fisher et
al., 2001
). Shear stress depends directly on volume flow
(Goldsmith and Turitto, 1986
).
When major alterations occur in one of the hemodynamic parameters that
directly influence the shear stress, altered expression of
shear-stress-responsive genes with secondary effects on cardiac development
can be expected. Other studies have also shown that alterations in
hemodynamics can precede the onset of structural defects
(Stewart et al., 1986
). The
marked decrease in mean blood flow observed in this study may lead to an acute
decrease in shear stress, which could be responsible for the induction of
cardiac malformations by altering shear-stress-responsive gene expression.
In summary, we conclude that obstruction of the right lateral vitelline vein results in major hemodynamic changes during the first 5 h after clipping. We suggest that these hemodynamic changes induce cardiovascular malformations by altering normal patterns of shear-stress-responsive gene expression.
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Acknowledgments |
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References |
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