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Journal of Chinese Integrative Medicine ›› 2007, Vol. 5 ›› Issue (3): 287-297.doi: 10.3736/jcim20070312

• Original Experimental Research • Previous Articles     Next Articles

Effects of Chinese herbal recipe Weichang'an in inducing apoptosis and related gene expression in human gastric cancer grafted onto nude mice

Ai-guang Zhao1,2, Jin-kun Yang1, Sheng-fu You1, Ting Li1, Hai-lei Zhao1, Ying Gu1, Lai-di Tang1, Jia-xin Qiu1   

  1. 1 Department of Oncology , Longhua Hospital ,Shanghai University of Traditional Chinese Medicine , Shanghai 200032 ,China
    2E-institutes of Shanghai Municipal Education Commission , Shanghai University of Traditional Chinese Medicine , Shanghai 200032 ,China
  • Online:2007-05-31 Published:2007-05-15

Objective: To investigate the mechanism of Chinese herbal recipe Weichang'an (WCA) in inducing cell apoptosis of human gastric cancer grafted onto nude mice.Methods: The high performance liquid chromatography was used for monitoring the stability of WCA. A human gastric cancer cell line SGC-7901 grafted in nude mouse was used as the animal model. The mice were divided into untreated group and two experimental groups. Animals in the two experimental groups received either WCA over a 34-day period or 5-fluorouracil (5-FU) over a 6-day period starting at the 8th day after grafting. Animals in the untreated group received normal saline on an identical schedule. Animals were killed 41 days after being grafted. To assess the effect of the treatment on tumor, the tumor weight was determined by the electron balance immediately after the animals were killed. SP immunohistochemical method was used to detect the expression of proliferating cell nuclear antigen (PCNA) in grafts. Apoptotic indices (AI) of the tumor cells were examined by terminal deoxynucleotidyl transferase-mediated deoxyuridine triphosphate fluorescence nick end labeling (TUNEL) method. SP method was also used to detect the expressions of cleaved caspase-3, caspase-8 and caspase-9. SYBR green dye I real-time quantitative polymerase chain reaction (RT-PCR) was used to assess the related gene alterations in mRNA level. The expressions of phospho-Stat3 (Tyr705) and bcl-2 proteins were detected by using SP method.Result: Compared with the untreated group, tumor growth was significantly inhibited by treatment of WCA or 5-FU (P<0.01, respectively). The tumor inhibition rate in the WCA-treated group was 48.70% and that in the 5-FU-treated group was 60.10%. The average labeling index (LI) for PCNA in the WCA-treated group and 5-FU-treated group was significantly decreased as compared with that in the untreated group, respectively. The AI of human gastric cancer grafted in the nude mice detected by using TUNEL method was significantly increased to (9.72±4.51)% in the WCA-treated group, while it was (2.45±1.37) % in the untreated group. 5-FU-treated group was also found a significantly increased AI compared with the untreated group. The expressions of cleaved caspase-3 and caspase-9 in the WCA-treated group and 5-FU-treated group were significantly increased as compared with those in the untreated group. But caspase-8 showed no significant alteration either in the WCA-treated group or in the 5-FU-treated group. The expression levels of Stat3 (2 –ΔΔCT=0.16) and bcl-2 (2 –ΔΔCT=0.10) detected by using RT-PCR were lower in the WCA-treated group than those in the untreated group. The expressions of phospho-Stat3 (Tyr705) and bcl-2 in the WCA-treated group were significantly decreased as compared with those in the untreated group. Conclusions: Chinese herbal recipe WCA can inhibit gastric cancer cell SGC-7901 growth in vivo, induce gastric cancer cell apoptosis and suppress the cell proliferation. WCA induces apoptosis through the caspase-9 and caspase-3 pathway in vivo. Its mechanism might be involved in the down-regulation of Stat3 and bcl-2 genes.

CLC Number: 

  • R735

Figure 1

HPLC print of WCA"

Table 1

Sequences of primers for RT-PCR amplified genes"

Gene name UniGene cluster Primer Sequences (5'-3') Combining sites (bp) Amplifiers (bp)
Stat3 Hs.421342 forward CCTGGAGCAGCTCCATCAG 254 58
reverse AAACTGCCGCAGCTCCATT 311
Fas Hs.244139 forward GGCCCCTGTGTGAGTTGAGT 1 363 60
reverse GCAACCATCACTGCCCCTACT 1 422
Bcl-2 Hs.12677 forward TGTTGGCCGGATCACCAT 2 557 60
reverse TCCCCAATGATCAGGTCCTTT 2 616
Bax Hs.1959428 forward CCAAGGTGCCGGAACTGA 382 57
reverse CCCGGAGGAAGTCCAATGT 438
Bcl-xl Hs.102558 forward CATCAGGCATTCCCAGTACCA 335 59
reverse GGGTCAGAGTGCGGTCCTT 393

Table 2

Effects of WCA on gastric cancer cell SGC-7901 (ヌ±S,%)"

Group n PCNA TUNEL
Positive rate P Intense positiverate P Total positiverate P AI P
WCA-treated 8 35.73±6.01** 0.000 5 3.39±1.48* 0.015 5 39.03±7.37** 0.000 9 9.72±4.51** 0.000 7
5-FU-treated 9 37.86±16.50* 0.032 5 5.62±4.21 0.197 2 43.48±19.77* 0.040 6 5.74±1.75** 0.000 7
Untreated 8 53.48±9.34 8.78±5.43 62.26±13.80 2.45±1.37

Figure 2

PCNA expression in various groups of human gastric adenocarcinoma cell line SGC-7901 grafted onto nude mouse detected by immunohistochemical method (SP method, ×400)A: Untreated group; B: WCA-treated group; C: 5-FU-treated group. PCNA is predominantly localized at nuclei."

Figure 3

Apoptotic cells labeled in various groups of human gastric adenocarcinoma cell line SGC-7901 grafted onto nude mouse detected by TUNEL (×400)A: Untreated group; B: WCA-treated group; C: 5-FU-treated group."

Table 3

Effects of WCA on cleaved caspase-3, caspase-8 and caspase-9 of gastric cancer cell SGC-7901 (ヌ±S,%)"

Group n Cleaved caspase-3 (Asp 175) Cleaved caspase-8 (Asp 374) Caspase-9
Positive rate P Positive rate P Positive rate P
WCA-treated 8 5.20±2.26* 0.036 7 4.44±2.67 0.682 7 8.87±6.08** 0.008 6
5-FU-treated 9 4.73±1.76* 0.045 1 4.81±3.41 0.542 4 5.57±3.70* 0.025 5
Untreated 8 2.82±1.84 3.94±2.10 2.25±0.78

Figure 4

Cleaved caspase-3 (Asp 175) expression in various groups of human gastric adenocarcinoma cell line SGC-7901 grafted onto nude mouse detected by immunohistochemical method (SP method, ×400)A: Untreated group; B: WCA-treated group; C: 5-FU-treated group. Cleaved caspase-3 is predominantly localized at cytoplasm and pronuclear."

Figure 5

Cleaved caspase-8 (Asp 374) expression in various groups of human gastric adenocarcinoma cell line SGC-7901 grafted onto nude mouse detected by immunohistochemical method (SP method,×400)A: Untreated group; B: WCA-treated group; C: 5-FU-treated group. Cleaved caspase-8 is predominantly localized at cytoplasm."

Figure 6

Caspase-9 expression in various groups of human gastric adenocarcinoma cell line SGC-7901 grafted onto nude mouse detected by immunohistochemical method (SP method, ×400)A: Untreated group; B: WCA-treated group; C: 5-FU-treated group. Caspase-9 is predominantly localized at cytoplasm and pronuclear."

Table 4

Quantification of gene expression by RT-PCR assay"

Gene UniGene cluster Untreated WCA-treated
Stat3 Hs.421342 ΔΔCT 0 (n=3) 2.65 (n=4)
2–ΔΔCT 1 0.16 (0.11-0.24)
Fas Hs.244139 ΔΔCT 0 (n=4) 2.40 (n=5)
2–ΔΔCT 1 0.19 (0.11-0.32)
Bcl-2 Hs.12677 ΔΔCT 0 (n=4) 3.27 (n=5)
2–ΔΔCT 1 0.10 (0.06-0.17)
Bax Hs.1959428 ΔΔCT 0 (n=4) 1.80 (n=5)
2–ΔΔCT 1 0.29 (0.14-0.59)
Bcl-xl Hs.102558 ΔΔCT 0 (n=4) 2.21 (n=5)
2–ΔΔCT 1 0.22 (0.16-0.29)

Table 5

Effects of WCA on expressions of P-Stat3 and bcl-2 of gastric cancer cell SGC-7901 (ヌ±S,%)"

Group n P-Stat3 bcl-2
Positive rate P Intense Positiverate P Total Positive rate P Positive rate P
WCA-treated 8 35.93±12.67** 0.002 4 3.64±1.72** 0.002 3 39.57±13.31** 0.000 2 1.62±0.82** 0.000 6
5-FU-treated 9 36.95±27.21 0.073 2 4.38±3.62** 0.005 0 41.33±30.22* 0.024 3 7.72±5.31 0.936 4
Untreated 8 56.49±9.34 13.16±7.06 69.65±10.80 7.53±3.73

Figure 7

Phospho-Tyr705-Stat3 expression in various groups of human gastric adenocarcinoma cell line SGC-7901 grafted onto nude mouse detected by immunohistochemical method (SP method,×400)A: Untreated group; B: WCA-treated group; C: 5-FU-treated group. Phospho-Tyr705-Stat3 is predominantly localized at nuclei."

Figure 8

Bcl-2 expression in various groups of human gastric adenocarcinoma cell line SGC-7901 grafted onto nude mouse detected by immunohistochemical method (SP method,×400)A: Untreated group; B: WCA-treated group; C: 5-FU-treated group. Bcl-2 is predominantly localized at cytoplasm and nuclear membrane."

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