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Ultrastructure and molecular biological changes of chronic gastritis, gastric cancer and gastric precancerous lesions: a comparative study
Goang-Yao Yin, Wu-Ning Zhang, Xiao-Jing Shen, Yi Chen, Xue-Fen He
Goang-Yao Yin, Xiao-Jing Shen,
Xue-Fen He, Wuxi No.3 peoples hospital,
Wuxi 214041, Jiangsu Province, China
Wu-Ning Zhang, Yi Chen,
Department of National Microanalysis Center, Fudan University, Shanghai 200433,
Shanghai, China
Correspondence to: Dr.
Goang-Yao Yin, Wuxi No.3 peoples hospital, 230 Eastern Tonghhui Road Wuxi
214041, Jiangsu Province,China. yinyao@pub.wx.jsinfo.net
Received:
2002-10-04 Accepted: 2002-12-03
Abstract
AIM: To carry out a comparative study on
ultrastructure and molecular biological changes of chronic gastritis (CG),
gastric cancer (GC) aand gastric precancerous lesions.
METHODS:
By the use of histochemical staining, SEM with EDAX, TEM with EDAX, image
analysis technique, RIA and chemiluminescence method, gastric mucosa of 168
patients were synchronously analyzed in morphology, trace elements, DNA, cAMP,
SOD, 3H-TdR LCT and serum LPO were also done.
RESULTS:
The
incidence of epithelial nucleoplasmic ratio >1, lobulated nuclei,
inter-chromatin aggregation of granules, nucleolar hypertrophy, and the content
of DNA, Zn, Cu in nuclei and serum LPO of each group were showed as belows:
normal control group (0.0, 0.0, 6.7, 0.0, 12.6±2.7,
7.6±0.4,
58.4±0.3,
2.6±0.6),
CSG group (5.7, 2.9, 7.4, 2.9, 15.2±3.1,
8.1±0.5,
58.9±0.5,
4.2±0.7),
CAG group (31.3, 29.7, 45.3, 42.2, 16.5±3.1,
8.6±0.4,
59.3±0.5,
4.5±0.6),
CA group (100.0, 100.0, 72.2, 50.0, 30.7±8.2,
8.8±0.3,
59.5±0.4,
6.8±1.6),
ATP++group
(61.5, 38.5, 23.1, 38.5, 23.5±8.9,
8.3±0.4,
59.1±0.4,
5.1±1.2),
IM+++
ATP++group
(77.8, 55.5, 33.3, 44.4, 25.1±7.2,
8.4±0.5,
59.5±0.4,
6.5±1.1),
IM++++ATP++
group
(100.0, 100.0, 75.0, 62.5, 28.5±9.1,
8.9±0.5,
59.7±0.4,
7.6±0.7),
IMIIb
group
(100.0, 62.5, 75.0, 50.0, 27.3±10.3,
8.6±0.3,
59.5±0.4,
6.1±0.9);
whereas the content of Zn, Cu in mitochondria and cAMP, SOD in gastric mucosa,
and 3H-TdR
LCT of each group were showen as belows: normal control group (9.2±0.5,
58.3±0.3,
15.9±1.5,
170.5±6.1,
1079.7±227.4),
CSG group (8.6±0.5,
57.8±0.3,
14.6±1.8,
163.3±5.6,
867.3±240.5),
CAG group (8.3±0.4,
57.5±0.3,
13.4±1.8,
161.2±4.3,
800.9±221.8),
CA group (8.9±0.4,
57.1±0.3,
10.2±3.9,
152.2±3.8,
325.7±186.8),
ATP++
group
(9.1±0.4,
57.0±0.3,
12.4±1.8,
161.5±3.8,
642.9±174.3),
IM++++
ATP++group
(8.6±0.4,
56.9±0.3,
12.0±2.3,
152.2±2.5,
326.3±160.3),
IM++++ATP++
group
(8.5±0.3,
56.8±0.2,
10.4±0.9,
147.4±2.6,
316.1±170.7),
IMIIb
group
(8.6±0.3,
56.9±0.3,
11.9±1.9,
150.0±2.8,
318.9±145.8),
there were significant differences between groups (P<0.05-0.01).
CONCLUSION: There
was a significant difference between CG and GC in their ultrastructure and
molecular biology. Only on the condition of changes of internal environment in
combination with the harmful effect of external environment, chronic
atrophic gastritis can then develop into gastric cancer. Hence it might have
similar epithelial cell ultrastructure and molecular biological changes in ATP++,
IMIIb and cancer, hence there were similar patterns of occurrence,
development and transformation. Recognition of this trend might help to explore
problems of prevention and cure.
Yin GY, Zhang WN, Shen XJ, Chen Y, He XF.
Ultrastructure and molecular biological changes of chronic gastritis, gastric
cancer and gastric precancerous lesions: a comparative study. World J
Gastroenterol 2003; 9(4): 851-857
http://www.wjgnet.com/1007-9327/9/851.htm
INTRODUCTION
We conducted histochemical staining, detection of
cAMP, SOD and DNA of gastric mucosa of 168 patients with chronic gastritis (CG)
or gastric cancer (GC); SEM and TEM with EDAX were used to synchronously
determine ultrastructures and trace elements and image analysis technique was
used to determine nuclear DNA. 3H-TdR LCT and serum LPO were also
cared out. Following was the comparative study.
MATERIALS AND METHODS
Materials
168 patients definitely diagnosed as
suffering from CSG, CAG and GC were our subjects of study. According to "the
standards for the classification of chronic gastritis, for gastrofiberscopic
diagnosis and for histopathological diagnosis of atrophic gastritis"
gastric mucosa tissue slices underwent HE staining and ABPH2.5/PAS,
Hid/ABPH2.5 and HiD/ABPH2.5 histochemical staining. ATP
was classified into low-grade, middle-grade and heavy-grade and IM into IM Ia,
IM Ib, IM IIa, IM IIb. 68 cases were definitely
diagnosed as CSG, including 43 males, 25 females, average age 43 years, average
course of disease 4a, 26 cases without IM or ATP; 31 cases with concomitant or
solitary IM-19 cases low-grade, 10 cases middle-grade and 2 cases heavy-grade; 9
cases with solitary ATP-8 cases low-grade, 1 case middle-grade; 2 cases with IM
and concomitant ATP, IM and ATP were both middle-grade. 64 cases were definitely
diagnosed as CAG, including 37 males, 27 females, average age 47 years average
course of disease 6a, 3 cases without IM or ATP; 39 cases with concomitant
solitary IM (17 cases low-grade, 4 cases middle-grade and 18 cases heavy-grade);
8 cases with solitary ATP (2 cases low-grade, 6 cases middle-grade.) 14 cases
with IM concomitant ATP (12 cases middle-grade IM, 2 cases heavy-grade IM, 8
cases low-grade ATP, 6 cases middle-grade ATP). 36 cases were definitely
diagnosed as GC, including 22 males, 14 females, average age 52 years, average
course of disease, 2a, all with IM or ATP. 12 cases with solitary IM (6 cases
low-grade, 3 cases middle-grade, 3 cases heavy-grade); 7 cases with solitary ATP
(1 case low-grade, 6 cases middle-grade); 17 cases with IM concomitant ATP (5
cases middle-grade IM, 12 cases heavy-grade IM; 7 cases low-grade ATP, 9 cases
middle-grade ATP, 1 case heavy-grade ATP). Of the 45 healthy volunteers who
underwent gastroscopy and biopsy, 15 cases had basically normal gastric mucosa
tissues, including 6 males 9 females, average age 37, and they were referred to
as normal control (NC) group.
Methods
Under gastroscopy, three pieces of gastric
mucosa were taken from the focal and nonfocal areas in antral region and body of
stomach as specimens for section preparation, SEM, TEM, detection of DNA, cAMP
and SOD. Blood was taken for 3H-TdRLCT and LPO. For the observation of gastric
mucosa ultrastracture and determination of its trace elements[1-4],
501B SEM with 9100/60 EDAX was used to observe the three pieces of specimens of
each patient, under the direct vision of SEM, the EDAX probe automatically
detected the samples within 0.1-0.01 mm2 range all the elements under 12 in
atomic number and automatically calculated the weight percentage (WT%) of each
element in element series. 15 points were fixed in the three pieces of mucosa of
every patient to carry out 15 detections, and the average WT% of each element
was taken as its actual WT%. In every detection, 21 elements such as Na, Mg, Al,
Si, P, S, K, Ca, Fe, Cu, Zn, Ti, Cr etc were detected, and weight percentage
(WT%) of each element between elements of gastric mucosa was calculated.
By using EM430 TEM
with 9100/60 EDAX, three pieces of mucosa specimens of every patient were
magnified in unison by five magnifying powers (3 600, 7 200, 14 000, 19 000, 29
000) to randomly take the pictures of the panoramagram, local area and organelle
and to detect the atomic number percentage (AT%) of each nuclear and
mitochondrial element between trace elements[5-10]. After gastric
mucosa cell smear was stained by Feulgen staining, IBAS 2000 image analysis
technique was adopted to detect IOD, which is taken as the relative content of
nuclear DNA[7,8]. RIA was adopted to detect the content of gastric
mucosa cAMP (Pmol/g); chemiluminescence method was adopted to detect the
activity of SOD (u/g)[4]. 3H-TdRLCT. (Bq/L whole blood)
was carried out; thiobarbituric acid development process was adopted to detect
serum LPO (u mol/L)[4].
Statistical method
x2 and t test.
RESULTS
Histopathology of gastric mucosa
Between NC group. CSG group. CAG group and CA
group, there were significant differences in the incidence rate and degree of
different types of IM and ATP in glands propria of gastric mucosa (P<0.05-0.001,
Table 1). The surface of normal gastric mucosa was isolated by crisscross small
groves into many lesser gastric areas, assuming convolution shape (Figure 1). In
these areas, there were many gastric pits (the mouths of gastric glands), which
were shaped like craters. The concave walls had round or oval epithelial cells
of almost the same size. In CSG gastric mucosa there were scattered denatured,
diabrotic and necrotic exfoliated epithelical cells, on whose surface S-shape Helicobacter
pylori (HP) were found (Figure 2). Massive epithelial cells became diabrotic,
anabrotic and exfoliated forming micro ulcers. The ulcers spred out from their
centers, with adjacent cells crushed, destructed in irregular shapes and
arrangement. In CSG gastric mucosa, cyst was found accidentally (Figure 3), the
epithelial cells of crater walls were atrophic and denatured, of different sizes
and deranged; the cells became diabrotic and necrotic and had inflammatory cell
infiltration and the glands propria of the serious cases were shaped like grid
framework structure (Figure 4). The surfaces of the epithelial calls of IM
gastric mucosa were thickly coated, villi were invisible and the intercellular
boundaries were not clear (Figure 5). SEM was not able to definitely indentify
gastric mucosa ATP, but only able to distinguish whether cells were hyperplastic
or not. Degeneration, hyperplasia or cellular regeneration occured in gastric
mucosa. The hyperplastic cells are of different sizes and states and the active
memberanes were shaped like lesser tubercles (Figure 6, 7). The cells of gastric
cancer were different sizes and shapes, deranged, characterized by obvious
heteromorphic nature, conglobated and shaped like grapes or cauliflower. There
were nearby or basal infiltration, destruction and ulceration of cancer cells,
which have developed into ulcers.
Figure
1 Convolution shape of mucosa surface. ×320.
Figure
2 Degeneration, diabrosis, necrosis and
exfoliation of gastric mucosa epithelial cells. ×640.
Figure
3 Cysts of gastric mucosa. ×64.
Figure
4 Atrophic and denatured glands propria in
grid framework structure. ×320.
Figure
5 The surface of IM cells is thickly coated,
intercellular boundaries are not clear. ×1 250.
Figure
6 The hyperplastic cells are of different
sizes and states, the active membranes are shaped like lesser tubercles. ×320.
Figure
7 The hyperplastic cells are of different
sizes and states, the active membranes are shaped like lesser tubercles. ×640.
Figure
8 The cells of gastric cancer are conglobated
and shaped like grapes. ×320.
Figure
9 There is an increase in inter chromatinic
grandules densification, nucleolar grandules become thick nucleoli expand
with irregular margins. ×14 000.
Figure
10 Nucleolar margination. ×7 200.
Figure
11 Multi nucleoli. ×14 000.
Figure
12 Nucleolar division. ×14 000.
Figure
13 Intranuclear inclusion. ×14 000.
Figure
14 The densification of inter
chromatinic grandules. ×14 000.
The ultrastructure of gastric
mucosa epithelial cells
The mucous cells on epithelial cell surface
of relatively normal gastric mucosa were columna epithelial cells covering
endogastric surfaces and inside wall of gastric pit. Their free surfaces had
short micro villi; the mucous neck cells were distributed over the necks of
gastric glands, and on the tops of these cells were a few short thick micro
villi. Chief cells were distributed over the bodies and bottoms of gastric
glands; parietal cells were big and conic and their conical tops turned towards
gland cavities; the endocrine cells lied between chief cells and parietal cells
and they were small, and their nuclei are round or oval, the nuclei envelopes
are slightly bent, lobulated nuclei were few, the nucleocyotoplasmic ratio was
less than 1.
The nuclear
chromatins were scattered, or associated with nucleoli or along nuclear
perimeters. The light bright zones between heterochromatins in the nucleoli are
euchromatins; the nucleoli had high electron density without capsule.
Mitochondria were round or oval, scattering around nuclei. The mitochondria
consisted of outer membrane, inner membrane, outer ventricle, inner ventricle
and cristae. Crista, the inward folded inner membrane, was a hollow canal
leading to outer ventricle. Some mitochondrial cristae directly led to
cytoplasms. Cristae were generally in tabular arrangement, parallel to each
other and vertical to mitochondrial long axes. In cytoplasms were many parallel
rough surfaced endoplasmic reticuluas (RERs), secretory granules, well-developed
Golgi's bodies and scattered mitochondria. The free
surfaces of epithelial cells of CG gastric mucosa had dropped micro villi; the
intercellular space expanded and cell conjuctions decreased; the karyoplasmic
ratio of both ill-differentiated epithelial cells and IM cells was greater than
1, and lobulated nuclei increased; nucleolar granules became thick and nucleoli
expanded with irregular margins (Figure 9).
There occured
nucleolar margination (Figure 10), multinucleoli (Figure 11) and nucleolar
division (Figure 12). The obsolescent epithelial nuclei shrank and the
karyoplasmic ratio was still less; the heterochromatins lied densely around
nuclei; the electron density was low in the center of nuclei and nuclei were
loop in shape. (referred to as chromatin margination); the shrunk nuclei were
denticular, in which the electron density was moderately homogeneous and
chromatins were not found (referred to as chromatin homogenization). There were
mitochondrial swelling, hypertrophy, pyknosis, hyaline degeneration as well as
vacuolar degeneration. The deformed mitochrondrias were in C-shape or U-shape.
There were zigzag, longitudinal, sparse and pyknosis cristae, and deranged
cristas. There was an decrease in the number of mitochondrias and their cristae.
There were mitochondrial decreases in number, mitochondrial swelling, or crista
fragmentation, vacuolar degeneration, and RERs in circular arrangement; the
Golgi抯 bodies become atrophic and had lost their
typical structures; the cytoplasmic incretory granules decreased. There were
still greater epithelial cell changes in cancer cells of gastric cancer than in
cells of gastric mucosa of chronic gastritis, intranuclear inclusion appeared
(Figure 13).
There was an
increase in peri-chromatinic and interchromatinic granular densification (Figure
14). In euchromatins; there was a significant difference between CSG group and
CAG group in nucleolar margination and nucleolar looping (P<0.05-0.001,
Table 2, 3); between IM IIb group, ATP++ group, IM+++ATP++
group and IM++++ATP++ group, compared with NC group, CSG
group and CAG group, the difference was also significant (P<0.05-0.001,
Table 2, 3). There is no significant difference between IM++++ATP++
group, IM IIb group and CA group (P>0.05, Table 2, 3).
The biochemical assay in gastric
mucosa and serum
The content of nuclear Zn and Cu increased
progressively in the sequence of NC group, CSG group, CAG group and CA group;
the content of mitochondrial Zn and Cu decreased progressively in the same
sequence. There was significant differences between these groups (P<0.05-0.001,
Table 4). The content of Zn, Cu, cAMP and SOD in gastric mucosa decreased
progressively in the same sequence; the content of DNA increased progressively
in the above sequence. There were significant differences between these groups (P<0.05-0.001,
Table 5). The content of 3H-TdRLCT decreased in the sequence of NC
group, CSG group, CAG group and CA group; content of serum LPO increased in the
same sequence; there was significant difference between these groups (P<0.05-0.001,
Table 6). Between IMIIb group, ATP++ group, IM+++ATP++
group and IM++++ATP++ group, NC group, CSG group and CAG
group, there was also significant difference (P<0.05-0.001, Table 4,
5, 6). Between IM++++ATP++ group, IM IIb group
and CA group, There was no significant difference (P>0.05, Table 4, 5,
6).
Table 1 Comparison between classification of IM and grading of ATP in CG and GC gastric mucosa n (%)
| Groups | n | IM classification | Grading of ATP | |||||||||
| Ia | Ib | IIa | IIb | ATP+ | ATP++ | IM+++ ATP+ |
IM+++ ATP++ |
IM++++ ATP+ |
IM++++ ATP++ |
IM++++ ATP+++ |
||
| NC | 15 | 2(13.3) | 1(6.7) | |||||||||
| CSG | 68 | 16(23.5) | 8(11.8) | 6(8.8) | 3(4.4) | 8(11.8) | 1(1.5) | 2(2.9) | ||||
| CAG | 64 | 16(25.0)b | 11(17.2)b | 13(20.3)d | 13(20.3)d | 2(3.1)d | 6(9.4)d | 7(10.9) | 5(7.8)c | 1(1.5) | 1(1.6) | |
| CA | 36 | 4(11.1) | 9(25.0)c | 16(44.4)df | 1(2.8)d | 6(16.7)d | 3(8.3) | 2(5.6)c | 4(11.1)f | 7(19.4)f | 1(2.8) | |
Either
Solitary IM or IM with concomitant ATP in CSG, CAG or CA is included in IM
classification statistically, compared with NC group. aP<0.05,
bP<0.01;
compared with CSG group. cP<0.05,
dP<0.01;
compared with CAG group. eP<0.05,
fP<0.01.
In table 2-6, the marks are the same as here.
Table 2 The ultrastructures of epithelial nuclei of gastric mucosa in CG and GC n (%)
| Group | n | Appearce | Chromatin | Nucleons | |||
| Nucleoplasmic ratio>1 | Nucleus lobulated | Margination or homogeneity | Perinuclcar concentrated |
Hypertrophy or margination | looping | ||
| NC | 15 | 1(6.7) | 1(6.7) | ||||
| CSG | 68 | 5(5.7) | 2(2.9) | 7(10.3) | 5(7.4) | 2(2.9) | 2(
2.9 |
| CAG | 64 | 20(1.3)d | 19(9.7)d | 33(51.6)bd | 29(45.3)bd | 27(42.2)d | 14(21.9) |
| CA | 36 | 36(00.0)bf | 36(00.0)bf | 17(47.2)d | 26(72.2)bdf | 18(50.0)d | 17(47.2)df |
| IMIIb | 8 | 8(100.0)b | 5(62.5)h | 5(62.5)b | 6(75.0)b | 4(50.0) | 3(37.5) |
| ATP++ | 13 | 8(61.5)hi | 5(38.5)hj | 4(30.8)bgj | 3(23.1)bhj | 5(38.5) | 1(7.7)hj |
| IM+++ATP++ | 9 | 7(77.8)hhik | 5(55.5)hk | 3(33.3)bgj | 3(33.3)bhj | 4(44.4) | 3(33.3)l |
| IM++++ATP++ | 8 | 8(100.0)ln | 8(100.0)jkm | 5(62.5)bkm | 6(75.0)blm | 5(62.5)lm | 3(37.5)l |
Compared
with CA group, gP<0.05,
hP<0.01,
Compared with IMIIb
group, iP<0.05,
jP<0.01,
Compared with ATP++
group, kP<0.05,
lP<0.01.
Compared with IM+++ATP++
group, mP<0.05,
nP<0.01.
In table 3-6, the marks are the same as here.
Table
3
Mitochondria utrastructures of gastric mucosa epithelial cells in CG and
GC (x±s)
| Group | n | Number | Swelling or Ovegrowth (%) | Matrix fading (%) | Vacuolar degeneration (%) | Pyknosis(%) | Crista number | Fragmentation and derangement of cristas(%) |
| NC | 15 | 86.5±27.3 | 3.4±1.6 | 3.0±1.1 | 2.9±1.9 | 1.1±0.8 | 12.8±3.2 | 2.2±1.1 |
| CSG | 68 | 65.4±21.1b | 7.2±3.8b | 7.8±5.0b | 6.4±4.5b | 1.9±0.9b | 8.2±3.2b | 5.8±3.1b |
| CAG | 64 | 52.2±20.8bd | 10.9±4.5bd | 11.7±8.6bd | 11.6±7.7bd | 3.7±1.1bd | 6.9±3.5bc | 8.9±3.7bd |
| CA | 36 | 38.8±31.5bde | 12.9±4.2bde | 15.6±5.4bdf | 14.6±5.8bde | 3.9±0.6bd | 8.1±1.9bde | 10.5±2.7bde |
| IMIIb | 8 | 36.8±30.8b | 13.8±3.2b | 14.1±4.3b | 12.5±3.9b | 3.3±0.8bg | 9.3±2.1b | 7.6±1.1bh |
| ATP++ | 13 | 49.1±27.9b | 11.3±2.9b | 8.3±3.5bh | 9.3±4.7b | 1.9±0.5bhj | 11.3±1.8hi | 5.2±1.2bhj |
| IM+++ATP++ | 9 | 41.3±30.8b | 12.8±2.1b | 12.1±2.8bg | 11.2±3.7b | 2.3±0.3bhjk | 11.0±1.5ahi | 6.2±1.3bhi |
| IM++++ATP++ | 8 | 35.4±31.5b | 13.3±4.3b | 15.2±5.3bl | 12.8±4.3b | 3.9±0.5bbln | 8.4±2.1bln | 8.6±1.0bhln |
Table 4 Nuclear and mitochondriaL Zn, Cu of gastric mucosa in CG and GC (x±s)
| Group | n | Nuclear | Mitochondria | ||
| Zn (AT%) | Cu(AT%) | Zn (AT%) | Cu(AT%) | ||
| NC | 15 | 7.6±0.4 | 58.4±0.3 | 9.2±0.5 | 58.3±0.3 |
| CSG | 68 | 8.1±0.5b | 58.9±0.5b | 8.6±0.5b | 57.8±0.3b |
| CAG | 64 | 8.6±0.4bd | 59.3±0.5bd | 8.3±0.4bd | 57.5±0.3bd |
| CA | 36 | 8.8±0.3bde | 59.5±0.4bde | 8.9±0.4bde | 57.1±0.3bde |
| IMIIb | 8 | 8.6±0.3b | 59.5±0.4b | 8.6±0.3b | 56.9±0.3b |
| ATP++ | 13 | 8.3±0.4bhi | 59.1±0.4bhi | 9.1±0.4i | 57.0±0.3b |
| IM+++ ATP++ | 9 | 8.4±0.5bg | 59.5±0.4bk | 8.6±0.4bl | 56.9±0.3b |
| IM++++ATP++ | 8 | 8.9±0.5bl | 59.7±0.4b | 8.5±0.3bgl | 56.8±0.2bh |
Table
5
Gastric mucosa Zn, Cu, DNA, cAMP and SOD
in CG and GC (x±s)
| Group | n | Zn (WT%) | Cu(WT%) | DNA(IOD) | cAMP(pmol/g) | S |
| NC | 15 | 4.1±1.0 | 5.2±0.8 | 12.6±2.7 | 15.9±1.5 |
