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Abstrak :
Objective: Cancer is a disease that gets serious attention in the medical world. This is due to the ever increasing number of patients and there has been no effective way to treat. Cancer cells have telomerase activity is relatively high compared to normal cells, so the cancer cells have the ability to continue to proliferate. Cancer cells undergo uncontrolled mitosis and have high telomerase activity compared to cells normal. Telomerase is an enzyme responsible for telomere length, a segment of DNA that is the tip of chromosomes in eukaryotic cells. Telomeres are associated with the process of aging and carcinogenesis. The purpose of this study was to determine the expression of telomerase in some cells such as breast cancer, cervical cancer, and lung cancer. Methods: The research method is experimental studies in several cancer cell cultures in the form of cell line. Cancer cells used were: HeLa (cervical cancer), MCF7 and T47D (breast cancer), WiDr (lung cancer), and Raji (lymphoma) with culture medium RPMI, DMEM, and M199. Vero cells is used (fibroblast cells) as a control (normal cells). Expression of telomerase enzyme was measured by the Immunohystochemistry (IHC) method. Results: The results showed that the cancer cells have activity/higher telomerase expression were highly significant (p<0.01) compared to normal cells (Vero cells). Similarly, the expression of telomerase in HeLa versus WiDr, WiDr versus T47D, T47D versus Raji, and Raji versus MCF7 also showed highly significant differences (p < 0.01). Telomerase expression between cancer cells that showed significant difference (HeLa cells versus Raji cells; HeLa cells versus MCF7 cell; T47D cells versus MCF7 cells) (p < 0.05). No significant difference was found in the group of HeLa cells versus T47D, WiDr versus Raji cells, and WiDr versus MCF7. Conclusions: It was concluded, that the cancer cells have telomerase expression of specific and different from each other, depending on the type of cell. T47D breast cancer cells have telomerase expression of the highest, followed by cervical cancer cells (HeLa). Lung cancer cells (WiDr) with cell lymphoma (Raji) has almost the same expression and both have lower expression.;

Abstrak :
Objective: Cancer is a disease that gets serious attention in the medical world. This is due to the ever increasing number of patients and there has been no effective way to treat. Cancer cells have telomerase activity is relatively high compared to normal cells, so the cancer cells have the ability to continue to proliferate. Cancer cells undergo uncontrolled mitosis and have high telomerase activity compared to cells normal. Telomerase is an enzyme responsible for telomere length, a segment of DNA that is the tip of chromosomes in eukaryotic cells. Telomeres are associated with the process of aging and carcinogenesis. The purpose of this study was to determine the expression of telomerase in some cells such as breast cancer, cervical cancer, and lung cancer. Methods: The research method is experimental studies in several cancer cell cultures in the form of cell line. Cancer cells used were: HeLa (cervical cancer), MCF7 and T47D (breast cancer), WiDr (lung cancer), and Raji (lymphoma) with culture medium RPMI, DMEM, and M199. Vero cells is used (fibroblast cells) as a control (normal cells). Expression of telomerase enzyme was measured by the Immunohystochemistry (IHC) method. Results: The results showed that the cancer cells have activity/higher telomerase expression were highly significant (p < 0.01) compared to normal cells (Vero cells). Similarly, the expression of telomerase in HeLa versus WiDr, WiDr versus T47D, T47D versus Raji, and Raji versus MCF7 also showed highly significant differences (p < 0.01). Telomerase expression between cancer cells that showed significant difference (HeLa cells versus Raji cells; HeLa cells versus MCF7 cell; T47D cells versus MCF7 cells) (p < 0.05). No significant difference was found in the group of HeLa cells versus T47D, WiDr versus Raji cells, and WiDr versus MCF7. Conclusions: It was concluded, that the cancer cells have telomerase expression of specific and different from each other, depending on the type of cell. T47D breast cancer cells have telomerase expression of the highest, followed by cervical cancer cells (HeLa). Lung cancer cells (WiDr) with cell lymphoma (Raji) has almost the same expression and both have lower expression.

Abstrak :
Pertumbuhan kanker tidak hanya ditentukan oleh adanya sel kanker itu sendiri akan tetapi ditentukan juga oleh lingkungan mikro disekitarnya. Lingkungan mikro tersebut merupakan jaringan yang heterogen dengan adanya interaksi sel termasuk sel punca mesenkim. Sekretom mengandung faktor-faktor biologis terlarut yang dapat mempengaruhi pertumbuhan sel kanker. Stem cell from Human Exfoliated Deciduous SHED diketahui merupakan sumber sel punca yang memiliki banyak potensi. Sampai saat ini belum diketahui bagaimana dampak pemberian CM dari SHED terhadap sel punca kanker payudara. Oleh karena itu, penelitian ini bertujuan untuk menganalisis pemberian conditioned medium kultur SHED pada sel punca kanker payudara terhadap viablitas, proliferasi dan tumorigenitas serta kepuncaan dari sel punca kanker payudaraALDH dan sel punca kanker MCF7. Conditioned medium SHED SHED-CM adalah medium kultur bebas serum sel SHED yang dikumpulkan dalam 24 jam dan 48 jam. ALDH dan MCF7diberikan 50 v/v SHED-CM 24 jam dan 48 jam dan di inkubasi selama 72 jam. Hal yang sama dilakukan untukperlakuan aktivasi CM dengan suhu. CM sebelum digunakan terlebih dahulu dipanaskan dalam suhu 80 C selama 10 menit. Kontrol adalah sel yang diberikan 50 v/v a-MEM. Perhitungan viabilitas sel dilakukan dengan menggunakan metode Trypan Blue Exclusion Assay dan ekspresi relatif mRNA dari TGF-b1, TGF-b1 receptor TBRI , ALDH1A1 dan OCT4 menggunakan qRT-PCR dan analisis menggunakan perhitungan livak. Hasil penelitian menunjukkan bahwa ekspresi relatif dari TGF-b1, TGF-b1 reseptor TBRI , ALDH1A1 dan OCT4 pada sel ALDH dan MCF7 pasca induksi dengan CM SHED mengalami peningkatan yang signifikan dibandingkan dengan kontrol. Selain itu, peningkatan yang lebih signifikan ditunjukkan pada perlakuan aktivasi dibandingkan yang tidak diaktivasi. Hal yang berbeda pada hasil uji viabilitas sel. Viabilitas sel mengalami penurunan pasca induksi dengan CM SHED sedangkan setelah diinduksi dengan CM SHED yang telah diaktivasi, viabilitas sel mengalami peningkatan yang signifikan pada sel ALDH dan MCF7. Dengan demikian sekretom SHED dapat meningkatkan viabilitas dan proliferasi serta kemampuan kepuncaan dari ALDH dan MCF7.

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Cancer development is not only determined by corresponding of cancer cells but also by the microenvironment. This includes a heterogen network of interacting cell include mesenchymal stem cells. Conditioned medium of MSC culture containing soluble factor hes been identified to affect intercellular communicating between MSC and cancer cells which could affect the stemness of cancer cells. Many studies reported that Stem cells from human exfoliated deciduous teeth SHED as a novel stem cell source with multipotent potential. However, the effect of MSC interaction with cancer cells can not be clearly understood so that the effects of safety in its utilization are not yet known for certain. This study is to confirm the relation between secretom of MSC from SHED with the stemness and agresiveness of ALDH and MCF7. SHED conditioned medium SHED CM , SHED were grown in serum free a MEM for 24 and 48 hours, consist of two groups, non heated and heated at 80 C for 10 min. Human BCSCs ALDH cultured in DMEM F12 were supplemented with 50 v v CM SHED 24 h and 48 h, as well as with heated by 72 h incubation. Control was BCSCs supplemented with 50 v v a MEM. We measured the viability with trypan blue assay and mRNA expression of TGF b1, TGF b1 receptor TBRI , as well as stemness genes ALDH1A1 and OCT4 using qRT PCR. The relative mRNA expression levels of TGF b1, T RI, OCT4 and ALDH1A1 in BCSCs supplemented with non heated SHED CM were increased compared to their control and also after TGF b1 heat activation was significantly higher than in non heated SHED CM. In the other hand, the viability cell was significantly reduced after supplemented with non heated SHED CM, but increased higher than control when treated with heated SHED CM, there are may be a role of the TGF b1 signaling involvement of other factors in SHED CM affect cell proliferation and increase the stemness. We found that secretomes SHED can increase proliferation of breast cancer stem cells ALDH and also expression of stemness gene OCT4 and ALDH1A1. the activation with heated can enhance the increase of proliferation and stemness. We assumed that signalling of TGF can affect tumor proggresion of ALDH and MCF7

Abstrak :
Kanker payudara merupakan jenis kanker yang sering terjadi pada perempuan di seluruh dunia. Saat ini baku emas diagnosis kanker payudara, yaitu pemeriksaan histopatologi, masih memiliki kekurangan dan bergantung pada penilaian visual pemeriksa. Penelitian ini dilakukan dengan menggunakan alat Direct Scanning Calorimetry (DSC) untuk mengidentifikasi profil termal pada sel kanker payudara. DSC sangat sensitif terhadap perubahan suhu yang kecil terkait aktivitas molekuler didalam sel. Penelitian ini dilakukan secara uji in vitro dengan menggunakan sel MCF7 sebagai sampel percobaan. Sel kanker dibagi menjadi kelompok tanpa dan dengan perlakuan doxorubicin dan sel normal payudara sebagai pembanding. Tiap kelompok diuji 4 kali pengulangan. Sel dilisis dan diambil 10 μL untuk dibaca profilnya menggunakan DSC-60. Hasil pemindaian DSC berupa termogram yang kemudian dianalisis dan didapatkan data nilai titik lebur dan entalpi lebur tiap sampel. Data diuji statistik menggunakan uji ANOVA satu arah. Termogram DSC sel MCF7 menunjukkan adanya 1 puncak fase transisi dengan titik lebur pada suhu 142,47 ± 7,908 oC dan entalpi lebur sebesar 1,61 ± 0,257 kJ/g. Hasil uji statistik menunjukkan perbedaan bermakna profil termogram sel MCF7 terhadap sel payudara normal dan sel MCF7 yang telah diterapi doxorubicin. DSC dapat digunakan sebagai alat untuk mengidentifikasi profil termogram sel MCF7. Profil termogram sel MCF7 yang dihasilkan memiliki karakter khas dan dapat dibedakan dengan sel payudara normal dan sel MCF7 yang telah diterapi doxorubicin. ...... Breast cancer is the most common type of cancer on women around the world. At present, the gold standard for the diagnosis of breast cancer, which is histopathological examination, still has some deficiencies and rilies on visual judgement. This research was conducted to utilize the Direct Scanning Calorimetry (DSC) as a tool to identify thermal profiles of breast cancer cells since DSC is very sensitive to small temperature changes due to intracellular activity. MCF7 cell line used as experimental samples. Cancer cells divided into groups without and with doxorubicin treatment and normal breast cells used as a comparison of cancer cells. Cells lysed and used as much as 10 μL each to be scanned using DSC-60. Test ran as much as 4 times for each group. DSC thermograms analyzed so that the data obtained for the value of melting point and enthalpy of each sample. The data tested statistically by one way ANOVA. Thermogram of MCF7 cells showed 1 peak transition phase. The results of the analysis showed that the transition phase had a melting point at a temperature of 142,47 ± 7,908 oC and a melting enthalpy of 1.61 ± 0.257 kJ/g. Statistical test results showed a significant difference of thermogram of MCF7 compare to normal cells and MCF7 treated with doxorubicin. This study showed that DSC can be used as a tool to identify the thermogram profile of MCF7 cells. The thermogram profile has a distinctive character and can be distinguished from normal breast cells and treated MCF7 cells.