|
Angioplasty and local delivery. Standard PTCA
equipment was used. An 8F right Amplatz guiding catheter
and right Judkin's guiding catheter were used for coagulation
of the left and right coronary arteries, respectively. Heart
rate, blood pressure and the electrocardiogram were monitored
throughout the experiment. Coronary angioplasty was performed
with a balloon size chosen to correspond to a balloon/artery
ratio of 1.1:1.2. Three 30-s inflations at 10 arm were performed
with a 30-s interval between inflations. All three coronary
arteries of each animal were subjected to PTCA.
After PTCA,
each animal's coronary artery was randomized to receive
either 600 ug BE
locally, vehicle alone locally or PTCA
only. The chemicals BE
and its vehicle 2-hydroxypropyl-beta-cydodextrin (HPCD)
were purchased from Sigma Chemicals. The InfusaSleeve catheter
(LocalMed, Inc., Palo Alto, California) was used for local
delivery (9). Five milliliters of the
designated substance was delivered at a driving pressure
of 10 arm and support balloon pressure of 6 atm. The dose
of BE
(~30 ug/kg body weight) was chosen as representative of
a daily dose of systemic BE
therapy used in previous studies, which ranges from 10 to
100 ug/kg.
Of the 18 animals, two died a few days after PTCA and were
excluded; thus, 16 animals were analyzed. Twelve animals
were euthanized at 28 days and four at 7 days. After premedication
and anesthesia, the right internal jugular vein and common
carotid artery were cannulated. After crossclamping
of the descending thoracic aorta through a left lateral
thoracotomy, exsanguination was performed, with simultaneous
administration of 1 liter of 0.9% sodium chloride solution.
The heart was perfusion-fixed in vivo with 2 liter of 10%
buffered formalin at 200 mm Hg, removed from the animal
and placed in 10% buffered formalin solution. The site of
PTCA was identified in relation to adjacent side branches,
which served as landmarks. The injured segment was harvested
with a 1-cm normal segment proximal and distal to the injured
site. Serial sections 3 to 5 mm long were made from the
harvested segment, with a minimum of at least three sections
(maximum of 5) from each PTCA site. The sections were stored
in buffered 10% formalin and dehydrated with increasing
concentrations of alcohol, followed by treatment with xylene
and paraffin. Each section was cut into 6-um-thick slices
with a microtome (Olympus cut 4060 E) and stained with Verhoeff's
stain for morphometric analysis.
Morphometric analysis. Measurements were made with
a video microscope linked to a 486 personal computer and
customized software. A minimum of three sections for each
injured segment were analyzed, and the results were averaged.
When individual values were widely discrepant for an injured
segment (observed in only one injured vessel), all sections
demonstrating rupture of the internal elastic lamina (IEL)
were included for analysis. Analyses were performed by an
examiner who had no knowledge of the treatment assignment
of the injured segments. The areas of external elastic lamina
(EEL),
IEL
and lumen were measured by digital planimetry, neointimal
area (IEL
- lumen area) and medial area (EEL
- IEL
area) were obtained. The fracture length ( FL)
was measured as the length of discontinuity of the injured
IEL,
and measurement of the extent of injury was controlled by
standardization for each artery, expressed in relation to
the circumference of the IEL
(10,11). The extent of injury was determined by the ratio
of FL
to IEL
circumference ( FL/IEL).
The percent neointima was defined as the percent total
vessel area occupied by the neointima ([intimal area/EEL]
X 100). Morphologic percent stenosis was calculated
as 100 (1 - lumen/IEL
area) (10). The restenotic index was
defined as [intimal area/ (intimal area + medial area)]/( FL/IEL
circumference) (11). Injury score
was determined as previously defined (12).
Immunohistochemistry. After slicing with a microtome
and blocking of nonspecific antibodies, the sections were
treated with mouse anti-proliferating cell nuclear antigen
(PCNA) antibodies and diluted biotinylated goat antimouse
antibodies. They were incubated with avidin-biotin (Elite
ABC Kit, Vector Laboratories, Burlingame, California), developed
with 3,3'-diaminobenzidine (Vector Laboratories) and counterstained
with hematoxylin. Porcine liver cells served as the positive
control. For each section, a 6-um slice counterstained with
hematoxylin without treatment with the primary antibody
(mouse anti-PCNA) served as the negative control.
Immunohistochemistry was performed on samples from animals
euthanized at seven days. The percentage of proliferating
SMCs was obtained by dividing the number of PCNA-positive
SMCs by the total number of SMCs in each field; separate
measurements were made for neointimal and medial layers.
To standardize comparison among treatment groups, measurements
were obtained at four fixed locations separated by 90°
for each section, and the results were averaged. For each
segment, two sections demonstrating a maximal neointimal
response were analyzed, and the results averaged.
Statistical analysis. Values are expressed as the
mean value ± SEM. Kruskal-Wallis analysis was used
for comparison of data among the three groups. Multiple
comparisons between the BE
and PTCA-only
groups and between the vehicle-only and PTCA-only
groups were made using the Student-Newman-Keuls test. Chi-square
analysis was used for comparison of proportions. Values
were considered significant at p < 0.05.
Table 1. Morphometric Analysis
| Characteristics |
BE |
PTCA
Only |
Vehicle
Alone |
p Value |
|
| Segnents
analyzed (n) |
12
|
9
|
10
|
NS
|
| Artery
size (mm) |
2.86
± 0.1
|
2.94
± 0.08
|
2.94
± 0.13
|
NS
|
| Balloon/artery
ratio |
1.22
± 0.03
|
1.2
± 0.02
|
1.17
± 0.03
|
NS
|
| EELref/EELinj |
1.01
± 0.05
|
1.16
± 0.11
|
1.31
± 0.15
|
NS
|
| Fracture
length (mm) |
1.64
± 0.27
|
1.71
± 0.25
|
1.81
± 0.25
|
NS
|
| Extent
of injury |
0.25
± 0.04
|
0.25
± 0.04
|
0.25
± 0.04
|
NS
|
| Neointimal
area (mm2) |
0.40
± 0.09
|
0.88
± 0.20
|
1.14
± 0.33
|
<0.05
|
Neointimal
area/fracture
length (mm2) |
0.25
± 0.04
|
0.5
± 0.07
|
0.58
± 0.13
|
<0.005
|
| Perecnt
neointima |
12.16
± 2.57
|
23.02
± 3.97
|
25.46
± 4.73
|
<0.025
|
| Neointima/media
area |
0.59
± 0.14
|
1.67
± 0.43
|
1.75
± 0.41
|
<0.01
|
| Percent
stenosis |
15.67
± 3.22
|
27.51
± 4.39
|
30.34
± 5.40
|
<0.025
|
| Restenotic
index |
1.3
± 0.14
|
2.4
± 0.23
|
2.42
± 0.22
|
<0.005
|
| Injury
score |
1.64
± 0.1
|
1.7
± 0.14
|
1.77
± 0.15
|
NS
|
|
|
EELref
= proximal reference segment external elastic
limina area; EELinj = injured segment
external elastic lamina area (averaged).
Data are presented as the mean value ±
SEM.
BE = 17-beta-estradiol;
NS = not significant
|
|
RESULTS
After PTCA and local delivery, the animals were allowed
to recover and gained weight steadily. Two animals died
48 and 72 h, respectively, after the procedure and were
excluded; thus, 16 animals were studied. Autopsy of the
two animals revealed occlusive thrombus at the site of PTCA
(in the BE-treated
vessel in one pig and in the vessel treated with PTCA only
in the other pig).
No changes in heart rate, electrocardiographic variables
or blood pressure were observed during local delivery.
Injured segments. The balloon/artery ratio and artery
diameter were similar among the three treatment groups (Table
1). Segments with intact IEL
in which discernible injury was absent were excluded from
analysis (two from the PTCA-only
group and one from the vehicle-only group). Two segments
were lost during harvesting (one from the vehicle-only group
and one from the PTCA-only
group).
Morphometric analysis. On morphometric analysis
at 28 days, arterial segments treated with local delivery
of BE
showed significantly less neointimal hyperplasia compared
with the other two treatment groups (Fig.
1). This beneficial effect was noted in all of the variables
of neointimal response to injury analyzed (Table
1). The extent of injury was similar among the three
groups, suggesting that the use of the InfusaSleeve catheter
was not associated with enhanced risk of injury. The noninjured
segments proximal and distal to the sites of PTCA
appeared morphologically normal, with no evidence of inflammation
or necrosis.
To exclude the existence of an inhibitory effect on intimal
proliferation due to the vehicle, analyses were performed
comparing segments treated with vehicle alone and PTCA
only, which showed no significant differences. In contrast,
significantly less intimal hyperplasia was observed in BE
treated segments as compared with segments treated with
PTCA
only (Fig. 2). Compared with PTCA
only or vehicle alone, BE
decreased neointimal formation by ~50%.
The existence of a significant protective effect of BE
as compared with placebo or vehicle treatment by gender
was then assessed (Table 2 and 3).
Although the extent of injury in the BE-treated
segments appeared slightly greater in males and slightly
less in females, compared with the other two treatment groups,
they were not statistically significant. A significant protective
effect of BE
on the neointimal response to injury was demonstrated in
both genders.
There were no significant differences in the effect of
BE
in the different arteries treated (left anterior descending
vs. circumflex vs. right coronary artery). Neointimal area
(0.28 ± 0.16 vs. 0.47 ± 0.16 vs. 0.46 ±
0.15 mm2, p = NS), neointimal area/ FL
(0.17 ± 0.04 vs. 0.35 ± 0.11 vs. 0.25 ±
0.06, p = NS) and restenotic index (1.2 ± 0.14 vs.
1.72 ± 0.27 vs. 1.12 ± 0.25, p = NS) were
similar in the different arteries treated with BE.
Immunohistochemistry. A statistically significant decrease
in proliferating SMCs
(PCNA-positive
SMCs)
was seen in the arterial segments treated with BE.
Among the different groups, the percentage of PCNA-positive
SMCs
in the neointima were 0.43 ± 0.26% with BE,
4.26 ± 1.17% with PTCA
only and 4.27 ± 1.37% with vehicle alone (p <
0.05 for BE
vs. other two groups). There were no significant differences
in the percentage of PCNA-positive
SMCs
in the media between the three groups: 0.4 ± 0.15%,
1.38 ± 0.87% and 1.24 ± 0.79% for BE,
PTCA
only and vehicle alone, respectively (p = NS).
Vascular remodeling. To determine the effect on
vascular remodeling of the agents used, the EEL
areas of the injured segment and of the normal vessel proximal
to the PTCA
site were obtained, and their ratio calculated (10).
No significant difference between the groups was noted:
1.01 ± 0.05, 1.16 ± 0.11 and 1.31 ±
0.15, respectively, for BE,
PTCA
only and vehicle alone (p = NS).
DISCUSSION
The present study demonstrates, for the first time, to
our knowledge, that locally delivered BE
decreases neointimal proliferation after PTCA
in pigs. The study also shows that
local delivery of BE
can be performed safely using the InfusaSleeve catheter,
without significant additional injury.
Table 2. Morphometric Data in
Male Pigs
| Characteristics |
BE |
PTCA
Only |
Vehicle
Alone |
p Value |
| |
| Extent
of injury |
0.32
± 0.05
|
0.26
± 0.04
|
0.26
± 0.04
|
NS
|
| Neointimal
area (mm2) |
0.51
± 0.13
|
1.01
± 0.29
|
0.99
± 0.23
|
NS
|
Neointimal
area/fracture
length (mm2) |
0.25
± 0.06
|
0.52
± 0.09
|
0.5
± 0.08
|
<0.025
|
| Neointima/media
area |
0.78
± 0.21
|
2.05
± 0.69
|
1.65
± 0.4
|
0.05
|
| Restenotic
index |
1.24
± 0.21
|
1.84
± 0.27
|
1.92
± 0.31
|
<0.025
|
|
|
Data are presented as the mean value ±
SEM.
Abbreviations as in Table 1.
|
|
Table 3. Morphometric Data in Female
Pigs
| Characteristics |
BE |
PTCA
Only |
Vehicle
Alone |
p Value |
| |
| Extent
of injury |
0.14
± 0.01
|
0.24
± 0.08
|
0.21
± 0.07
|
NS
|
| Neointimal
area (mm2) |
0.25
± 0.07
|
0.73
± 0.3
|
1.51
± 1.05
|
NS
|
Neointimal
area/fracture
length (mm2) |
0.25
± 0.13
|
0.46
± 0.11
|
0.77
± 0.41
|
<0.05
|
| Neointima/media
area |
0.33
± 0.07
|
1.23
± 0.43
|
1.99
± 1.16
|
NS
|
| Restenotic
index |
1.37
± 0.2
|
2.75
± 0.38
|
2.93
± 0.43
|
<0.05
|
|
|
Data are presented as the mean value ±
SEM.
Abbreviations as in Table 1.
|
|
Local delivery and injury response. Systemic administration
of pharmacologic agents may not achieve a local concentration
of the agent to produce a significant effect; in addition,
higher doses may result in intolerance or toxicity. Unlike
systemic administration, local delivery involves the delivery
of a single dose of the agent during PTCA.
Therefore, local delivery appears to be a potentially effective
method for the prevention of tissue response to injury.
Several agents have shown beneficial results in reducing
neointimal proliferation after PTCA
in animal experiments. Locally delivered ethanol (13),
nitric oxide (10), vascular endothelial
growth factor (14) and antisense oligonudeotides
(15) have resulted in decreased neointimal
proliferation after arterial injury. Two clinical trials
have demonstrated that local radiation therapy may have
the potential to reduce restenosis after PTCA
(1,2).
17-Beta-estradiol and injury response. Previous
experiments in animals have demonstrated that estrogen administered
subcutaneously for up to three weeks inhibited the myointimal
response to arterial injury (7,8).
Recently, a preliminary report has suggested that short-term
subcutaneous estrogen therapy (6 to 17 days) may be effective
in reducing the injury response (16).
Estrogen administered intramuscularly for at least three
weeks has also demonstrated the potential to inhibit vascular
SMC
proliferation and neointimal hyperplasia (17).
However, the efficacy of local delivery of BE
to inhibit intimal hyperplasia has not been previously studied.
In the present study, local delivery of BE
was associated with a markedly lower proliferatioe response
compared with the other two treatment groups. The neointimal
area, neointima/media area ratio, restenosic index and morphologic
percent stenosis were all significantly lower in the BE-treated
arterial segments. The decreased neointimal hyperplasia
after treatment with BE
is probably due to the inhibition of SMC
proliferation. Assessment at different time points could
possibly provide additional information on the effect of
BE
on SMC
proliferation. Studies examining SMC
proliferation after arterial injury have shown that maximal
SMC
proliferatioe activity occurs during the first seven days
after experimental arterial injury and rapidly decreases
beyond seven days (18). We were able
to demonstrate significantly lower SMC
proliferation at seven days in the arterial segments treated
with BE,
compared with the PTCA-only
and vehicle-only treatment groups. The inhibitory effect
of BE
on SMC
proliferation may be due to a direct effect on SMC
proliferation (19) or to enhanced
synthesis of nitric oxide by BE
(20,21). Nitric
oxide is known to inhibit both SMC
migration (22) and proliferation (23).
The biologic effects of estrogen, like other steroid hormones,
involve intracellular receptors (24).
Estrogen receptors have been demonstrated in coronary arteries
obtained from autopsy specimens in both premenopausal and
postmenopausal women (25) and in cell
cultures of human saphenous vein and internal mammary artery
specimens (26). The beneficial effects
of BE-the predominant circulating estrogen in premenopausal
women-on vascular injury response may not be replicated
by other kinds of estrogens. For example, conjugated equine
estrogen was found to have no effect on neointimal proliferation
in nonhuman atherosclerotic primate models (27).
In this study, it is unlikely that loss of estrogen receptors
in the hypercholesterolemic monkeys could be responsible
for the lack of response to conjugated equine estrogen on
neointimal proliferation, as conjugated equine estrogen
treatment did result in a statistically significant decrease
in atherosclerotic plaque area and inhibited the progression
of atherosclerosis (with no effect on neointimal proliferation)
in the same monkeys, thereby demonstrating responsiveness
to estrogen. Simultaneous administration of progesterone
may attenuate the vascular injury response to BE
(28). A sexually dimorphic response
to estrogen has been reported after arterial injury, with
intact male rats deriving no benefit from estrogen therapy
(29). However, this sexually dimorphic
effect was not observed in another experiment with gonadectomized
rats (8). In the present study, a significant
effect of BE
on the neointimal proliferatioe response was noted in both
genders, although the male animals used in the study had
been castrated at birth.
Vehicle. 17-Beta-estradiol is a lipophilic compound
with poor solubility in aqueous solutions; therefore, it
needs a vehicle for parenteral administration. 2-Hydroxypropylbeta-cyclodextrin,
a starch derivative, has been successfully tested as an
effective excipient for protein drugs (30).
The pharmacokinetics of HPCD
are similar to that of insulin, and the toxic dose (nephrotoxicity)
has been estimated to be 200 mg/kg in rats (31).
The dose of HPCD
used to dissolve BE
in the present study was 0.63 mg/kg, far below the toxic
dose. Furthermore, HPCD
has been used for administration of ophthalmic preparations
and intravenous anesthetic agents in humans (32,33).
In the present study, the neointimal response to injury
was similar in HPCD-treated
arteries and arteries undergoing PTCA
only. Therefore, HPCD
itself did not exert any significant influence on neointimal
proliferation.
Clinical evidence. Retrospective studies in humans
have shown no benefit of hormonal replacement therapy on
angiographic restenosis after PTCA
(34), although one study did show
a beneficial effect after directional atherectomy (35).
However, conjugated estrogen (and not BE)
was the predominant form of estrogen used in many of these
patients, and no information on concomitant use of progesterone
is available. In addition, it is not known whether hormone
replacement therapy could achieve a sufficient concentration
of estrogen locally at the PTCA
site to exert a significant response.
Study limitations. It is possible that spillover
of BE
into the systemic circulation could occur during local delivery.
Also, tissue uptake and retention of BE
after local delivery were not measured. However, the results
of the morphometric and immunohistochemical analyses dearly
demonstrate a significant difference in the arteries treated
with BE
compared with untreated vessels, which is highly suggestive
of an effect due to the locally delivered BE.
The efficacy of the InfusaSleeve catheter in delivering
various agents intramurally has been reported in previous
studies. At a support balloon pressure similar to that used
in the present study, a sixfold higher concentration in
the arterial wall was achieved by local delivery, as compared
with the arterial wall concentration achieved by systemic
administration (36).
In another study, persistent retention in the arterial wall
of locally delivered tissue factor pathway inhibitor was
demonstrated for at least 48 h after delivery (37).
A strong argument against a systemic effect due to spillover
is that, in the present model, where all three treatment
arms were applied in each animal, the systemic effects of
BE
(if any) due to spillover would be expected to affect all
three coronary arteries in each animal equally, providing
equal protection to all vessels. The differences in the
results between the arteries treated with BE
compared with PTCA
only and vehicle alone cannot therefore be attributed to
such systemic effects. Furthermore, BE
that enters the circulation is rapidly eliminated, mostly
by the liver (38).
Conclusions. We have shown that a single dose of
BE
delivered locally during PTCA
in a porcine model has the potential to decrease neointimal
hyperplasia significantly, probably by inhibition of SMC
proliferation. Previous studies have demonstrated that treatment
with BE
is associated with inhibition of proliferation of human
vascular SMCs
in cell culture assays (6). The local
delivery of BE
can be performed safely with the InfusaSleeve catheter,
without risk of additional injury. The local administration
of BE
is therefore a promising new approach that may be useful
in preventing the proliferative response after PTCA.
Its usefulness in preventing restenosis after PTCA
merits further investigation.
Acknowledgments
The authors are indebted to Pascale Geoffroy, MSc, and Julie
Lebel for assistance in the laboratory; to Martin G. Sirois,
PhD, Dominique Lauzier and Veronique Philibert for assistance
with immunohistochemistry and morphometry; and to Stanley
Nattel, MD, FACC, for his valuable suggestions in the manuscript
preparation.
Reprint requests and correspondence: Dr. Jean-Francois
Tanguay, Montreal Heart Institute, Research Center, 5000
Belanger Street East, Montreal, Quebec, Canada HIT 1C8.
E-mail: tanguay@icm.umontreal.ca.
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