Tyrosol, a phenylethanoid and a derivative of phenethyl alcohol, possesses various biological properties, such as anti-oxidative and cardioprotective activity. Olive oil is the principal source of tyrosol in the human diet. However, so far the anti-cancer activity of tyrosol has not yet been well defined. This study therefore undertakes to examine the cytotoxic activity and the mechanism of cell death exhibited by tyrosol in KB human oral cancer cells. Treatment of KB cells with tyrosol induced the cell growth inhibition in a concentration- and a time-dependent manner. Furthermore, the treatment of tyrosol induced nuclear condensation and fragmentation of KB cells. Tyrosol also promoted proteolytic cleavage of procaspase-3, -7, -8 and –9, increasing the amounts of cleaved caspase-3, -7, -8 and –9. In addition, tyrosol increased the levels of cleaved PARP in KB cells. These results suggest that tyrosol induces the suppression of cell growth and cell apoptosis in KB human oral cancer cells, and is therefore a potential candidate for anti-cancer drug discovery.

β-carotene is present in carrots, pumpkins, and sweet potatoes. It suppresses many types of cancers by regulating cellular proliferation and apoptosis through a variety of mechanisms. However, the effects of β -carotene on oral cancer cells have not been clearly established. The main goal of this study was to investigate the effects of β-carotene on cell growth and apoptosis in oral cancer cells. Our results demonstrate that treatment with β-carotene induced inhibition of cell growth, and that the effect was dependent on β-carotene treatment time and concentration in KB cells. Furthermore, treatment with β-carotene induced nuclear condensation and fragmentation in KB cells. β-carotene promoted proteolytic cleavage of procaspase-3, -7, -8 and –9 with associated increases in the concentration of cleaved caspase-3, -7, -8 and –9. In addition, the level of cleaved PARP was increased by β-carotene treatment in KB cells. These results suggest that β-carotene can suppress cell growth and induce apoptosis in KB human oral cancer cells, and that it may have potential usefulness in anti-cancer drug discovery efforts.

Bacillus thuringiensis subsp. aizawai KB098 (이하 KB098 균주)은 파밤나방에 높은 살충 활성을 보인다. 해충에 살충 활성을 나타내는 내독소 단백질은 cry gene에 의해 발현이 되는데 cry gene은 주로 Bacillus thuringiensis의 plasmid DNA 상에 존재한다. KB098의 plasmid DNA를 추출하여 PCR을 수행한 결과, Cry1Aa, Cry1Ab, Cry1C, Cry1D 총 4개의 cry gene을 가지고 있는 것으로 확인되었다. KBM-1은 KB098균주를 curing한 mutant 균주로, KB098균주를 42℃조건에서 48시간 배양하고, UV를 조사하여 확보하였다. KBM-1의 plasmid DNA를 PCR한 결과 KB098에서처럼 Cry1Aa, Cry1Ab, Cry1C, Cry1D의 cry gene이 증폭됨을 알 수 있었다. KBM-1은 KB098처럼 crystal을 암호화하는 plasmid DNA를 가지며, cry gene을 보유하고 있다. 반면 KB098과는 달리 KBM-1 균주는 내독소 단백질을 생성하지 못하며 파밤나방의 생물 활성 검정에서 독성을 나타내지 않았다. 이러한 원인을 밝히고자 KBM-1 plasmid DNA의 특정 cry gene의 PCR 결과, 증폭된 cry 유전자 내에서 염기서열의 변화에 기인할 것이란 가정하에, KB098과 KBM-1 균주의 특정 plasmid DNA 상에서 증폭된 cry gene의 염기서열을 비교분석 할 것이다. 이를 통해 crystal 형성에 관여하는 유전자의 변이 유무를 확인할 계획이다.

Cruciferous vegetables including diindolylmethane (DIM) have been shown to have anticancer activity. Especially, DIM-pPhBr and DIM-pPhF used in this study was reported to have more effective and less toxic effects than DIM. However, there is no report presenting their anti-tumorigenic activity in oral cancer. In the present study, we examined the effects of DIM-pPhBr and DIM-pPhF on the cell proliferation and apoptosis in KB human oral cancer cells. DIM-pPhBr and DIM-pPhF decreased cell proliferation and induced apoptosis evidenced by western blot analysis, DAPI staining and sub-G1 population. This provides the first evidence that DIM-pPhBr and DIM-pPhF originating from cruciferous vegetables induce apoptotic cell death in human oral cancer cells to inhibit cancer cell proliferation.

Bacillus thuringiensis(B.t.)에서 cry gene은 plasmid DNA상에 존재하고 대상 곤충에 살충활성을 나타내는 내독소단백질 형성에 관여하는 주요 유전자이다.파밤나방(spodoptera exigua)에 높은 살충활성을 보이는 B.t. subsp. aizawai KB098 균주의 cry gene이 위치하는 plasmid DNA를 찾기 위해 curing 방법을 사용하였다. KB098균주는 cry1Aa, cry1Ab, cry1C, cry1D 4개의 cry gene을 가지고 있으며, Plasmid DNA는 7개가 확인되었다. Cry gene을 암호화하는 plasmid DNA를 찾기 위한 curing 방법은 LB배지에 KB098균주를 희석 후, 27℃ 진탕배양기에서 24시간 배양한 뒤 NA배지에 spreading 한 후, 42℃조건으로 48시간 배양하여 단일 colony를 얻었다. 위상차현미경으로 관찰했을 때 내독소단백질을 형성하지 않는 colony를 NA배지에 streaking하여 27℃ 조건으로 4일간 배양하였다. 위상차현미경관찰을 통해 내독소단백질을 형성하지 않는 colony를 선발하였다. Curing과정이 제대로 수행되었는지 확인하기 위해 SDS-PAGE를 통하여 분자량 130kDa의 내독소단백질 band가 형성되지 않음을 확인하였으며, PCR증폭을 통해 acrystalliferous균주가 KB098 균주가 가지고 있는 4개의 cry gene을 가지고 있지 않음을 확인하였다. cry gene을 암호화 하는 plasmid DNA를 찾기 위해 KB098균주와 5개의 acrystalliferous균주와의 plasmid DNA pattern을 비교하였다. acrystalliferous균주에서 결실된 plasmid DNA만을 gel elution 한 후에 PCR을 통해 cry gene의 존재를 확인하였다.

Tannic acid가 파밤나방의 중장액에 존재하는 단백질분해효소의 활성을 저해함으로 처리된 Bacillus thuringiensis(이하 B. thuringiensis) subsp. kurstaki KB100균주의 insecticidal crystal proteins(ICPs)의 과분해를 억제하며 살충활성을 상승시키는 효과가 있다는 연구결과를 기초로, tannic acid의 protease inhibition여부 및 tannic acid가 B. thuringiensis KB100균주의 parasporal inclusion에 미치는 영향을 조사하였다. Tannic acid와 파밤나방 중장액을 먼저 혼합하여 반응시킨 후 B. thuringiensis KB100의 parasporal inclusion에 처리하여 SDS-PAGE를 통해 단백질밴드를 확인한 결과, 중장액내의 단백질분해효소에 의해 정상적으로 분해되어 60KDa의 살충활성을 나타내는 독소단백질 밴드를 나타냈다. 따라서 tannic acid에 의한 살충활성증대의 정확한 영향을 확인하기 위해, B. thuringiensis의 parasporal inclusion과 먼저 혼합하여 반응시킨 후 파밤나방 중장액을 처리하고 단백질 밴드패턴을 확인한 결과 전독소인 130kDa의 단백질이 거의 분해되지 않고 나타났다. B. thuringiensis KB100의 parasporal inclusion과 tannic acid을 먼저 혼합하여 반응시킨 것을 위상차현미경하에서 확인한 결과, tannic acid의 농도가 높아질수록 parasporal inclusion이 응집하여 있는 것이 확인되어, tannic acid가 파밤나방 중장 내 소화효소에 반응하는 영향보다 B. thuringiensis 독소단백질의 응집을 통해 소화효소의 분해저해 원인 가능성을 확인하였다.

Betulinic acid (BA), a naturally occurring triterpene found in the bark of the white birch tree, has been investigated to induce apoptosis in various cancer cells and animal models. However, there is no report of the chemopreventive effect of BA in cervical cancer cells. Using KB human cervical cancer cells as a model, we currently show that BA decreases cell viability and induces apoptotic cell death. The mechanism of the BA-induced anti-growth response in KB cells is due to the down-regulation of specificity protein 1 (Sp1) and its downstream targets, myeloid cell leukemia-1(Mcl-1) and survivin. Thus, BA acts as a novel chemopreventive agent through the regulation of Sp1that is highly expressed in tumors.

MspTL is the major surface protein of Treponema lecithinolyticum associated with periodontitis and endodontic infections. Our recent investigation revealed that MspTL induces proinflammatory cytokines and intercellular adhesion molecule 1 in THP-1 cells and periodontal ligament cells. In this study we conducted oligonucleotide microarray analysis to investigate the global transcriptional regulation in THP-1 cells stimulated with purified recombinant MspTL. MspTL upregulated the expression of 90 genes in THP-1 cells at least four fold, and the functions of these genes were categorized into adhesion, apoptosis/antiapoptosis, cell cycle/growth/differentiation, chemotaxis, cytoskeleton organization, immune response, molecular metabolism, proteolysis, signaling, and transcription. The majority of the modified genes are known to be NF-κB-responsive and interferon-stimulated genes (ISGs). The expression of 12 selected genes was confirmed by real-time RT-PCR. Because prostaglandin E2 (PGE2) is an important inflammatory mediator and Cox-2 was found to be induced by MspTL in the microarray analysis, we determined the level of PGE2 in the culture supernatants of MspTL-treated cells and found that MspTL significantly increased PGE2. Our results provide insight into the gene regulation of host cells in response to MspTL, and may contribute to the understanding of the molecular mechanism in periodontitis.

cry gene은 Bacillus thuringienesis(B.t.)에서 대상 곤충에 살충활성을 나타내는 내독소단백질을 형성하는 주요 유전자로 특정 plasmid DNA상에 암호화되어 있 다. B.t. subsp. aizawai KB098 균주는 파밤나방(spodoptera exigua)에 높은 살충 활성을 보이는 균주로 본 연구에서는 이 균주의 cry gene이 위치하는 plasmid DNA를 찾고자 하였다. 본 실험에 이용된 KB098균주는 cry1Aa, cry1Ab, cry1C, cry1D 4개의 cry gene을 가지고 있으며, Plasmid DNA는 7개가 확인되었다. Cry gene을 암호화하는 plasmid DNA를 찾기 위해 acrystalliferous균주가 필요하였으 며, 42℃조건으로 48시간 열처리 후 새로운 배지에 27℃ 조건으로 3일간 재배양 하여 sporulation단계에서 위상차현미경관찰을 통해 내독소단백질을 형성하지 않 는 colony를 autolysis 단계까지 배양한 후에 위상차현미경으로 재확인하여 확보 할 수 있었다. 획득한 14개의 acrystalliferous를 균주 중, 서로 다른 pattern의 plasmid DNA를 갖는 5개의 균주를 선발하였고, acrystalliferous재확인을 하기 위 해 SDS-PAGE를 통하여 내독소단백질의 분자량인 130kDa의 band가 형성되지 않음을 확인하였으며, PCR증폭을 통해 acrystalliferous균주가 KB098 균주가 가 지고 있는 4개의 cry gene을 가지고 있지 않음을 확인하였다. cry gene을 암호화 하는 plasmid DNA를 찾기 위해 KB098균주와 선발한 5개의 균주와의 plasmid DNA pattern을 비교한 결과, 두 개의 plasmid DNA band에서의 차이가 확인되 었다.

This study aims to reveal how EA affects BAX and NF-kB involved in cell deaths from global ischemia, and to do this, observes the changes of BAX and NF-kB caused by EA application after transient global ischemia. The experimental method is to give rise to global ischemia and apply EA to 27 SD rats with the particulars of being six-week-old, male, around-300 gram-weighing, and adapted to laboratory environment for more than a week, and divide them into three groups, that is, GV20 EA group(n=9), L14 EA group(n=9), no-treatment GI group(n=9), and then observe their changes of BAX and NF-kB at the time lapse of 6 hours, 9 hours and 12 hours after ischemia, using western blotting. The numerical decrease of BAX expression at the time lapse of 9 hours after EA application, though not statistically significant, was observed in GV20 EA group and L14 EA group, and the NF-kB expression appeared statistically significant decrease in GV20 EA group and L14 EA group, but the expression was higher in the group with EA application. Therefore, EA application at the early phase of global ischemia is considered to affect BAX and NF-kB and play a positive role in decreasing apoptosis and cell deaths by inflammation.

Bacillus thuringiensis subsp. kurstaki KB100 isolated from the domestic soil have the most effective activity against the beet armyworm, Spodoptera exigua larva. The tannic acid as protease inhibitor might be increased the efficacy of sublethal concentrations of B. thuringiensis. The tannic acid was identified as a protease inhibitor that could increased the efficacy of sublethal concentrations of B. thuringiensis. Mixture of B. thuringiensis and tannic acid was investigated the mortality of S. exigua larva in the laboratory and field. When B. thuringiensis treated to 2nd larva of S. exigua, mortality was shown 54.4%. However, mixtures of B. thuringiensis with 4 and 40 mM tannic acid were increased mortalities to 2nd larva of S. exigua as 64.0 and 95.5%, respectively. Also, synergy effect of mixture of B. thuringiensis and 40 mM tannic acid was increased the mortality of S. exigua 3rd larva to 93.3%, even though 60.0% mortality with only B. thuringiensis treatment. On the other hand, the mortality of mixture with B. thuringiensis and 80 mM tannic acid was 53.3% lower than B. thuringiensis single treatment. In the welsh onion field, the accumulated mortalities of 3 times replicated with mixture of B. thuringiensis and 40 mM tannic acid were 83.9, 89.4 and 66.8% compare with 61.8, 80.4 and 47.3% as only B. thuringiensis treatment, respectively.

Artemisia scoparia (A. scoparia), perennial herb is indigenous to Korea and has been traditionally used in liver damage. We investigated the effect of the essential oil obtained from A. scoparia on apoptosis of KB cells. Cytotoxicity and cellular DNA content were analyzed by MTT assay and flow cytometry, agarose gel electrophoresis, and Hoechst 33258 staining. The caspase-3 and poly (ADP-ribose) polymerase (PARP) proteins were estimated by Western blotting method. We found that the essential oil induced the apoptosis of the KB cells by concentrations of 0.4 to 0.2 mg/ml which was verified by DNA fragmentation, apoptotic bodies, and the sub-G0/G1 ratio. The essential oil also transient caspase-9 and caspase-3 activity and cleavage of PARP in KB cells for 24 h. The essential oil-induced apoptotic cell death was accompanied by up-regulation of Bax and down-regulation of Bcl-2. In conclusion, we demonstrated that the essential oil of A. scoparia induces apoptosis in KB cells

In the present study, we have demonstrated that a novel synthetic chemical JSH-21 of N¹-Benzyl-4-methylbenzene-1,2-diamine could inhibit nitric oxide (NO) production in lipopolysaccharide (LPS)-activated macrophages RAW 264.7. The JSH-21 showed an IC50 value of 9.2 uM on the LPS-induced NO production. Furthermore, JSH-21 attenuated LPS-induced mRNA and protein levels of inducible NO synthase (iNOS) in the cells, as well as inhibited LPS-induced iNOS promoter activity. These results indicates hat the compound could down-regulate iNOS expression at the transcription level. Since NF-kB activation is a key mechanism in the expression of LPS-inducible iNOS gene, we further examined whether JSH-21 could affect LPS-induced NF-kB activation. JSH-21 inhibited LPS-induced nuclear import of NF-kB p65 in macrophages RAW 264.7 and sequentially prevented NF-kB transcriptional activity. However, JSH-21 was not effective in a LPS-induced degradation of cytoplasmic IkB-alpha in the cells. These results suggest that JSH-21 could inhibit LPS-induced NF-kB activation targeting nuclear import of NF-kB, an event downstream IkB degradation. Taken together, this study may provide a pharmacological potential of JSH-21 in the NO- or NF-kB-associated inflammatory disorders.

Oral squamous cell carcinoma (OSCC) is the most common malignancy and is a major cause of worldwide cancer mortality. The proto-oncogene c-myb plays an important role in regulation of cell growth and differentiation, and it is expressed at high levels in hematopoietic cells and many other types of cancers. However, the function of c-myb is not well known in OSCC. The present study aimed to reveal the function of c-myb and to test the alternation of cell growth and signaling by c-myb in OSCC. In this study, c-myb and dominant-negatibe myb(DNmyb) were expressed in an adenovirus-mediated gene delivery system to KB cells. The over-expressed c-myb brought increased cellular proliferation compared with control cells. However, DN-myb infected KB cells showed significant reduction of cell growth and enhanced induction of apoptosis to activate PARP and caspase 9. c-myb induced increase of IGF-I, -II and IGF-IR expressions while DN-myb down-regulated these expression. Activation of ERK and Akt/PKB pathway was shown only in c-myb transduced cells. These findings suggest that the role of c-myb in cell growth of oral cancer cells is partially mediated through the modulation of IGFs, ERK and Akt/PKB. From this results, DN-myb is strongly recommended as a curable gene for the treatment of c-myb dependent malignancies such as OSCC.

Treatment of oral cancers with chemotherapeutic agents become evaluated as an effective method to reduce cancer cell proliferation. Anti-proliferative and anti-oral cancer activities of momordin I on oral cancer cells were evaluated in this study. Momordin I was originally purified from a natural product, Ampelopsis radix and showed the antiproliferative activity against oral carcinoma, KB cells. Obtained value was approximately 104μM/mℓ. Time-and dose-dependent chromosomal DNA fragmentations were observed in momordin I-treated KB cells. Flow cytometry analysis showed time-dependent apoptotic cell appearance after treatment of momordin I. Approximately 18.6% apoptotic cells were observed at 72 hours after of momordin I treatment. These observation were consistent with the results obtained in DNA fragmentation analysis. These data suggest that momordin I has anti-proliferative effect and induces cell death in KB cells through apoptosis.

Indirubin is the active ingredient 0 1' a traditional Chinese herbal medicine, Danggui Longhui Wan, used for the t reatment of chronic myelocytic leu kelma The author reports that novel indirubin derivative, 5'-nitro-indirubinox ime (5'-NIO) , has potent a nti -proliferative activity on human o1'al cancer cells , Treatment of KB cells with 5’ NIO s howed a s t rong cell growth inhibit ion during indicated time point , A typical apoptosis pattern was obtained with DNA fragmenta tion and i mmunofl uorescence analysis of annelxn-v-f!ous Western blot data revealed that p53 and p21CIP1/Waf- l level increased strongJy upon 5'-NIO treatment , The a uthor next tested whether 5'-NIO could activate apoptos is related proteins s uch as caspase-3/-7/-9, [n cells exposed to 5‘-NIO, activation of caspase-3 and -7 was observed, Interesti ngly‘ caspase-9 and cytochrome c cou ld s li ghtly activate in response to 5’-NIO. These results indicate that 5’-NIO strongly induces oral cancer cells apoptosis via a Mi tochondria-mediated cas pase cascade pathway, These observations together s uggest that 5’ NTO may have a possible therapeutic potentia[ to oral cancer