|
Jun-Gong
Zhao, Ming-Hua Li, Ying-Sheng Cheng, Department of Radiology,
Sixth Affiliated Hospital of Shanghai Jiaotong University, Shanghai
200233, China
Gan-Sheng Feng, Xiang-Quan Kong, Xin Li, Department of
Radiology, Union Hospital, Tongji Medical College, Huazhong
University of Science and Technology, Wuhan 430022, Hubei Province,
China
Correspondence to: Dr. Jun-Gong Zhao, Department of
Radiology, Sixth Affiliated Hospital of Shanghai Jiaotong
University, Shanghai 200233, China. zhaojun_gong@sohu.com
Telephone: +86-21-64369181 Ext 8882
Received: 2003-09-09
Accepted: 2003-10-22
Abstract
AIM: To observe the change of tumor microcirculation after
transcatheter arterial chemoembolization (TACE) with bletilla
microspheres by using first pass perfusion MR imaging (FP) and
Chinese ink casting.
METHODS: VX2 carcinoma cells were surgically implanted into the left
and right lobes of liver of 30 New Zealand white rabbits, which were
divided into 3 groups at random. Emulsion of lipiodol mixed with
mitomycin C, and 5-FU bletilla microspheres were injected
into the hepatic artery respectively, and saline was used as control
agent. MR imaging was performed with turbo-flash sequence 14 d after
tumor implantation and 7 d after interventional therapy. The
steepest slopes (SS) of the signal intensity versus time curves were
created for quantitative analysis, 7.5% Chinese ink gelatin solution
was injected through ascending artery (17 cases) or portal vein (2
cases) for lesion microvessel area (MVA) measurement after the last
MRI examination.The correlation between perfusion imaging and MVA
was studied blindly.
RESULTS:
The SS values at the rim of tumor in lipiodol group (mean, 49% per
second) and bletilla group (mean, 35% per second) were
significantly decreased (P<0.05) as compared with control
group (mean, 124% per second), no difference was found between
lipiodol and bletilla groups (P>0.05). In lipiodol
group, the MVAs (24 974±11 836 mm2)
in the center of the tumor were significantly smaller than those of
the control group (35 510±15 675 mm2) (P<0.05), while the MVAs (80 031±22
745 mm2)
around the tumor were significantly increased because small and
dense plexuses appeared around the tumor which correlated to intense
reaction of granulation tissue. None of the vessels was seen in the
tumor in bletilla group, the peripheral MVAs of the tumor
were significantly smaller than those of the control group (P<0.05)
and lipiodol group (P<0.05). There was a good correlation
between SS and MVAs in control group (rs, 0.985, P<0.0001)
and bletilla group (rs, 0.743, P<0.05),
the correlation was not significant in lipiodol group (rs,
0.527, P>0.05).
CONCLUSION:
TACE with bletilla microspheres may enhance its anti-tumor
effect by inhibiting the angiogenesis, and FP-MRI provides useful
information to assess the TACE effect by depicting tumor
vascularization and perfusion.
Zhao JG, Feng GS, Kong
XQ, Li X, Li MH, Cheng YS. Changes of tumor microcirculation after
transcatheter arterial chemoembolization: First pass perfusion MR
imaging and Chinese ink casting in a rabbit model. World J
Gastroenterol 2004;
10(10): 1415-1420
http://www.wjgnet.com/1007-9327/10/1415.asp
INTRODUCTION
Transcatheter arterial chemoembolization (TACE) has been widely
used and is considered to be an effective conservative treatment for
hepatocellular carcinoma[1,2]. Rapid development of small
vessels after TACE resulting in incomplete necrosis, however,
reduces therapeutic effectiveness[1-9]. Therefore,
inhibition of the development of arterial collaterals may be
important in enhancing the therapeutic efficacy of this treatment.
Recently, TACE with microspheres, microcapsules, cyanoacrylate and bletilla
has been shown to improve the therapeutic results[1,3,10-12].
Bletilla microspheres have also been shown to improve the
therapeutic results because of its embolization of the hepatic
artery and portal vein as well as controlled release systems,
although changes at the level of hepatic microcirculation are not
completely elucidated.
The purpose of this study was to observe the change of tumor
microcirculation after TACE with bletilla microspheres by
using first pass perfusion MR imaging (FP) and Chinese ink casting.
MATERIALS
AND METHODS
Animals and tumor models
The VX2 tumor model used in this study was initially a
virus-induced papilloma first seen in domestic rabbit in 1937. With
sequential transplantations, the tumor line became increasingly
anaplastic[13]. VX2 carcinoma (Department of Radiology,
Union Hospital, Tongji Medical College, Huazhong University of
Science and Technology, Wuhan, China) was retained for
approximately 4 years by repeated passage of tumor every
14-21 d by way of intramuscular or subcutaneous implantation into
the thighs of male New Zealand white rabbits.
Twenty-five
male and five female New Zealand white rabbits (Laboratory Center,
Tongji Medical College) weighing 1-1.5 kg were used. Prior to all
procedures, including tumor implantation and imaging, rabbits
received an intramuscular injection of 1.0 mL/kg of body weight of
ketamine hydrochloride injection (Shanghai Sino-west Pharmaceutical
Company), intravenous access was then acquired via a marginal ear
vein. Anesthesia was maintained by using the same dose of
intravenously administered ketamine hydrochloride.
The
technique for tumor implantation was basically similar to that
described by Li et al[14]. Briefly, the liver was
exposed by performing midline laparotomy, VX2 tumor fragments of
approximately 1 mm3 were injected intraparenchymally into
the right and left lobes of the rabbit liver. Thirty New Zealand
white rabbits with tumors were divided into three groups at random.
They were group A (control group, 8 rabbits), group B (lipiodol
group, 12 rabbits) and group C (bletilla
group, 10 rabbits). All three groups received their
interventional therapy 14-21 d after tumor inoculation when MRI
confirmed the successful implantation.
Interventional
therapy
A polyethylene catheter (inner diameter 0.3 mm, outer
diameter 0.5 mm) was retrogradely inserted into the gastroduodenal
artery, the following agents were manually injected into the
gastroduodenal artery, namely, saline only into group A, 0.4-0.6 mL
lipiodol (Aulnay Sous-Bios, France) emulsion (lipiodol mixed with
MMC) into group B, 0.3 mL ultravist mixed with 10 mg bletilla
microspheres (Department of Radiology, Union Hospital, Wuhan, China,
40-200 mm
in diameter, combined with 5-FU) into group C.
MR imaging and data analysis
Fourteen days after tumor implantation and 7 d after
interventional therapy, MR imaging was undertaken by using a 1.5 T
system (Magnetom Vision, Siemens Medical Systems) with a head coil.
Transverse spin-echo T1-weighted images (repetition time was 525 ms,
the echo time was 14 ms) and HASTE T2-weighted images (repetition
time was 4.4 ms, the echo time was 90 ms) were obtained by using a 3
mm thick section, 0.5 mm intersection space, and four signals were
acquired.
For the FP, a strongly T1-weighted, turbo-FLASH sequence was
used with a high temporal resolution of 1.196 s per section, a
single image was acquired sequentially with 65 repetitions, which
resulted in an acquisition time of 2 min. The repetition time was
3.3 ms, the echo time was 1.4 ms, and time interval was 300 ms. At
the end of the fourth acquisition, a dose of 0.1 mmol/kg body weight
of gadopentetate dimeglumine (Bellona, Beijing, China) was
administered via a marginal ear vein.
To
quantitatively analyze FP, four circular ROIs were hand drawn,
covering the center and rim of the lesion, signal intensity time
curve was obtained over ROIs, and the steepest slope of the curve
(SS) was calculated according to the previously described method[15].
Evaluation
of anti-tumor effect
Tumor
size was measured with calipers. The size of each tumor on the liver
surface was measured immediately before treatment and seven days
after treatment on MR imaging. We evaluated the anti-tumor effect
based on the tumor volume, which was calculated as follows: tumor
volume (mm3)=0.5×a×b2,
where a is the length of major axis and b is the length of minor
axis measured with calipers.
Chinese
ink casting and histological evaluation
The
tumor microvessels were demonstrated by perfusion of 75 g/L Chinese
ink (Beijing Chinese Ink Company) gelatin solution into the
ascending artery (17 cases) or portal vein (2 cases) after the last
MR imaging examination. Before perfused with 75 g/L Chinese ink
gelatin solution, 500 units of heparin was administered
intravenously. After the rabbits were killed, the livers were
removed and stored at -20 °C for 24 h. The
specimens were immersed in 250-995 mL/L ethyl alcohol at increasing
concentrations, and finally in a solution of methyl salicylate. When
the oil penetrated the tissue, the specimens became transparent. The
sections (50 mm)
were observed first under a low power microscope (×40), then the sections with most dense area of microvessels
were selected and observed under a high power (×200).
Micro-vessels filled with Chinese ink gelatin were evaluated under a
microscope, micro-vessel areas (MVAs) in the center and rim of the
lesion were calculated by an imaging analysis system (Beijing
Aeronautic University). A 5 mm
sections of the same specimens
were stained with hematoxylin and eosin for light microscopy.
Statistical
analysis
All
data were expressed as mean±SD,
the statistical differences between different groups were analyzed
by ANOVA, and the correlation between SS and MVA was assessed by
Spearman correlation analysis. Significance was accepted when P<0.05.
RESULTS
MR imaging
MR imaging depicted all tumors on pretreatment images. All
untreated tumors had a low signal intensity on T1-weighted images
and an intermediate signal intensity on T2-weighted images. Central
areas of high signal intensity on T2-weighted images and low signal
intensity on T1-weighted images were compatible with the central
necrosis when tumors were larger than 1 cm. T1-weighted images after
injection of gadolinium showed a slight enhancement in the center of
lesion and a rim enhancement around the center of lesion in all
tumors (Figure 1). No significant difference in tumor volume was
observed among the three groups before therapy.
Tumor volumes in the lipiodol group and bletilla group
after TACE were significantly decreased compared with the control
group on d 7 after treatment, no significant difference in tumor
volumes was observed between lipiodol group and bletilla
group (Figure 2, Table 1). The central slight enhancement area was
larger, and the peripheral arterial phase rim enhancement in the two
groups was thinner. The SS values at the rim of tumor in lipiodol
group (mean, 49% per second) and bletilla group (mean, 35%
per second) were significantly decreased (P<0.05), as
compared with the control group (mean, 124% per second), no
difference was found between lipiodol group and bletilla one
(P>0.05) (Table 2).
Table
1 Tumor volumes
pre- and post-treatment (cm3)
| Group |
Pre-treatment |
Post
treatment |
| Control |
0.430±0.067 |
1.620±0.327 |
| Lipiodol |
0.465±0.120 |
0.971±0.285a |
| Bletilla |
0.402±0.171 |
0.736±0.145a |
aP<0.05
vs control.
Table 2 SS
values at the rim of tumor in different groups
| Group |
SS
(%.s-1) |
F |
P |
| Control |
124±62 |
|
|
| Lipiodol |
49±15 |
11.08 |
0.004
a |
| Bletilla |
35±9 |
6.88 |
0.019
a |
aP<0.05
vs control.
Table 3 Correlation
between SS values and MVA in different groups
| Group |
SS
(%.s-1) |
MVA
(mm2) |
rs |
P |
| Control |
124±62 |
35
510±15
675 |
0.985 |
<0.05 |
| Lipiodol |
49±15 |
80
031±22
745 |
0.527 |
>0.05 |
| Bletilla |
35±9 |
15
530±7
973 |
0.743 |
<0.05 |
Figure
1(PDF) Images obtained before treatment in control
group. A: T1WI
shows hypointense lesions in left lobe of the liver. B:
T2WI shows homogeneous hyperintense lesions in left lobe of the
liver. C: FP
T1-weighted image with gadolinium shows rim enhancement and no
enhancement in the center of lesion. D: Signal intensity time curve
derived from FP, SS of the curve in the border of the lesion is
steeper than that of the normal liver.
Figure 2(PDF) Images obtained after treatment in lipiodol group.
Inhomogeneous hyperintense lesions with intermediate intense rim
(arrow head) can be seen on T1WI (A)
and T2WI (B),
indicating the necrosis of the lesion and intratumor retention of
lipiodol. (C) FP
T1-weighted image with gadolinium shows thinner rim enhancement and
no enhancement in the center of the lesion compared with control
group although the lesion volume is increased. (D) SS of the curve
in center of the lesion is decreased compared with those of the
border.
Chinese
ink casting
Investigation
under microscope (×40) of the livers filled with Chinese ink in control group
revealed networks of vessels or plexuses of dilated and tortuous
course around and within the tumor originated from the arterioles,
some sinusoid vessels were observed in the tumors, all these vessels
were clearly distinct from the lobular architecture. In lipiodol
group after TACE, the MVAs within the tumor (24 974±11
836 mm2)
were significantly smaller than those of the control group (35 510±15
675 mm2)
(P<0.05), while the MVAs around the tumor (80 031±22
745 mm2)
were significantly increased, as compared with the control group (35
510±15
675 mm2)
(P<0.05). Small and dense plexuses appeared around the
tumor, with unknown origin. None of the vessels was seen in the
tumor in bletilla group after TACE (Figure 3). The peripheral
MVAs of the tumor (15 530±7
973 mm2)
in bletilla group were significantly smaller than those of
the control group (35 510±15
675 mm2)
(P<0.05) and lipiodol group (80 031±22 745 mm2) (P<0.05).There
was a good correlation between SS and MVA at the rim of tumor in
control group (rs, 0.985, P<0.0001) and bletilla
group (rs, 0.743, P<0.05), the correlation was not
significant in lipiodol group(rs, 0.527, P>0.05) (Table
3).
Figure
3 Micro-vessel casting with Chinese ink through ascending
artery. A: The
specimens show a lobular architecture of normal liver, magnification
×100. B:
In control group, hepatic artery perfusion shows networks of
micro-vessels or plexuses of dilated and tortuous course around and
within the tumor originated from the arterioles, some sinusoid
vessels can be observed in this tumor, magnification ×100.
C: The original
micro-vessels of the tumor are remarkably diminished, small and
dense new plexuses appear around the tumor in lipiodol group, which
are correlated to intense reaction of granulation tissue,
magnification ×100.
D: micro-vessels
are decreased in bletilla group, no new micro-vessels can be
seen at all, magnification ×100.
Figure 4 Histological examinations of hepatic lesion before and after
treatment. A: HE
stain shows nidal arrangement of VX2 cells as well as micro-vessels
filled with Chinese ink before treatment, magnification ×200.
B: In lipiodol
group, histological examination shows coagulation necrosis at the
center of lesion, very few micro-vessels can be seen within this
zone, residual tumor cells are seen at the periphery of lesions,
moreover, an intense reaction of granulation tissue is seen within
this area, small dense vessels are scattered at border of the
lesion, and congested sinusoids are seen in the periphery of the
tumor, magnification ×200.
C: Coagulation
necrosis as well as large infarcts involving multiple adjacent
lobules is seen in bletilla group, few vessels are seen at
the border of the lesion, magnification ×200.
Pathologic
correlation
The specimens did not show necrosis or infarct when the
lesion was less than 1 cm in control group. In lipiodol group none
lesions underwent complete necrosis, coagulation necrosis was
demonstrated at the center of all lesions. Viable or residual
cancerous tissues as well as an intense reaction of granulation
tissue were seen at the periphery of all lesions in lipiodol groups
after TACE, small and dense vessels were scattered at the border of
the lesions, correlating with the irregular thick rim enhancement on
MR image. In bletilla group after TACE, all lesions
demonstrated complete coagulation necrosis, large infarcts involving
multiple adjacent lobules were seen as well, few vessels were seen
at the border of the lesion, no granulation tissue was seen (Figure
4).
DISCUSSION
Bletilla
inhibition of tumor micro-vessels
A
previous study reported an intense reaction of granulation tissue at
the periphery of all lesions in lipiodol group[16], the
dense angiogenic plexus in the granulation tissue is, to our
knowledge, a new finding. Granulation tissue which resulted in
capillary proliferation and permeability increase was correlated to
arterial phase rim enhancement on MR image. Angiogenesis was central
to tumor stroma formation and offered nutrition to the remaining
viable tumor cells, which limited lipiodol embolization and
anti-tumor effect. As a result, local tumor recurrence would occur
sooner or later[7-9,16].
TNP-470, cyanoacrylate and Plcg-mitomycin-microsphere have
been used to inhibit capillary networks or to prolong first-pass
effect and to enhance the anti-tumor effect of TACE[1,17-20].
Our experimental study indicated that bletilla could enhance
the anti-tumor effect of TACE as well. Bletilla, as an
anti-tumor and anti-inflammation agent, is a Chinese medicine[10,12].
Its microspheres (mixed with 5-FU, 40-200 mm
in diameter) can result in dual embolization (embolization of
hepatic arterial and portal venous blood supply) and inhibit the
microvessels around and in the tumor completely. The reason why no
microvessels developed after TACE was partly due to its anti-tumor
and anti-inflammation effect, partly through inhibition of the
binding of vascular endothelial growth factor to its receptor[10].
As a result, treatment with bletilla could necrose the tumor
thoroughly. This was why bletilla could enhance the
anti-tumor effect of TACE even the lesion was very large[12].
VX2
microcirculation morphology
Many materials, including Chinese ink and microfil, have
been used to demonstrate the vascular morphology of tumors[17,21].
Among them, microfil is commonly used because of its different
colors, which could identify the origin of vessels. But microfil was
too viscous to get into the sinusoid, no vessel was visible inside
the tumors less than 0.25 mm in diameter[17].So we
selected less viscous materials to reveal microvessel morphology of
VX2. Three percent of Chinese ink gelatin solution was used to
explore the vascular architecture of cheek pouch carcinoma[21].
To avoid overfilling the microvessels, we added gelatin to increase
the viscosity of the solution to obtain 7.5% solution. As a result,
all the microvessels of normal liver including arterioles and
sinusoid were filled with black Chinese ink, so did those of tumor.
Moreover, the pathologic change of the other part of the same
specimens stained with HE could be observed. So microvessel casting
correlating with pathologic change could assess the changes of tumor
microcirculation at the same time. We believe that Chinese ink
gelatin solution casting may be used as the golden standard to
evaluate the microvessels in perfusion study with CT and MR imaging.
Value of FP-MRI
Although power Doppler US has been used to assess
vascularity of tumors[23-25], before contrast enhanced
harmonic power Doppler US has widely been used, the major problems
in the use of power Doppler are as follows. The detected velocities
were too slow in the tumor, there were too many blooming artifacts
associated with micro-bubble injection, the duration of enhancement
was short and there were artifacts resulted from respiration[23].
So the vascularity of tumors could not be evaluated in detail by
power Doppler US. FP-MRI, with a high time resolution, can monitor
the contrast agent first passing the target tissue by using signal
intensity time curve, the steepest slope of which (SS, i.e. the
maximum upward slope of the curve) correlates linearly with flow
velocity and angiogenesis, and has been successfully used to
quantify the myocardial perfusion reserve and to depict the tumor
vascularization[15,22], but no study has assessed the
tumor microcirculation after TACE by FP[26,27]. Our
experimental result revealed that areas with the fastest contrast
medium uptake (SS) colocalized significantly with focal hot spots of
MVA in control group and bletilla group, but no significant
correlation was observed between SS and MVA in lipiodol group,
suggesting that factors beyond the MVA are involved in the
gadopentetate dimeglumine
-related signals
enhanced in microvessels. We believed that the discrepancy could
reflect the difference between small dense vessels newly developed
at the border of the lesion after lipiodol treatment and tumor
microvessels before treatment. The new vessels were hyperpermeable[28],
part of the small molecular contrast media (gadopentetate
dimeglumine) might leak out of microvessels even at first
pass course. On the other hand, the new vessels might be too small
to have the same flow velocity like those before treatment. So we
believed that when the same categoric vessels were assessed by FP,
the flow velocity might be constant, the SS was correlated linearly
with MVA. When different categoric vessels were evaluated by FP, the
flow velocity and permeability were different, and not dependent
only on MVA.
In
this study, bletilla microspheres were administered for 7 d
only, and further studies of extended duration are needed. We
conclude that tumor microvessels can be markedly inhibited by using bletilla
microspheres in combination with 5-FU, which can explain and confirm
its effectiveness in clinic. The SS derived from FP has a good
correlation with MVA and may be used as a noninvasive method to
quantitatively evaluate tumor angiogenesis after TACE.
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