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Abstrak :
Latar Belakang: Ekstrak jintan putih Cuminum cyminum memiliki potensi efektivitas antibakteri dan anti jamur serta tidak toksik terhadap sel fibroblas tikus. Belum terdapat penelitian yang meneliti toksisitas ekstrak jintan putih terhadap Dental Pulp Stem Cells DPSCs . Tujuan: Mengetahui efek ekstrak jintan putih konsentrasi 0,1 mg/ml, 0,4 mg/ml, 0,7 mg/ml, dan 1,0 mg/ml terhadap viabilitas DPSCs. Metode: Menggunakan uji MTT dengan menghitung nilai absorbansi menggunakan microplate reader, dengan hasil akhir berupa nilai optical density OD yang dipersentasekan terhadap kelompok kontrol. Hasil: Terdapat perbedaan viabilitas DPSCs yang bermakna ......Introduction The extract of cumin Cuminum cyminum has the potential antibacterial and antifungal activity and it was not toxic for mouse fibroblasts. However, there have been no research investigating the toxicity of cumin extract on Dental Pulp stem Cells DPSCs . Aims To compare viability DPSCs of Cuminum cyminum extract 0,1 mg ml, 0,4 mg ml, 0,7 mg ml, and 1.0 mg ml . Methods Cell viability was analyzed using MTT Assay by calculating absorbance value using microplate reader, with optical density OD as the final result. Results There were significant differences statistically in viability on DPSCs p

Abstrak :
Objective: To compare the importance of storage time and the tooth type for isolation of dental pulp cells (DPCs) from extracted human teeth. Methods: 35 human teeth were used in this study. The teeth were stored in phosphate buffered saline (PBS) after extraction and divided into two groups randomly according to the time elapsed between extraction and isolation. In group one, the isolation was performed within 2 hours and in the other group it was performed 24 hours after extraction. Results: No significant differences between isolation time and total cell counts (p 0.483) and between isolation time and viable cells (p 0.341). No significant differences between the first molar and the premolar related cell counts and viable cells, but both teeth groups showed significant higher viability and had higher total cell amounts than third molars after isolation. Statistically significant correlations were found between age of donors and viable cells and viability after 24 hours isolation time. Conclusion: The immediate isolation of DPCs is not necessary after the tooth extraction. The tooth can be stored in PBS at room temperature up to twenty four hours after the extraction without a significant reduction in cell viability and counts. The cells obtained from younger donors might have more chance for more viability even if storage time was extended. Premolars and first molars were better donors than the third molars for DPCs isolations and the high number of success revascularization rate in premolars with necrotic immature premolars might be because of their high cell viability potentials.

Abstrak :
Latar belakang: Celah bibir dan palatum atau cleft lip and palate (CLP) merupakan kelainan kongenital multifaktorial yang mengakibatkan pasien memiliki defek pada jaringan lunak dan keras di bagian bibir dan palatum. Pasien celah bibir dan palatum umumnya menderita gangguan estetik dan fungsi stomatognatik. Sehingga, untuk mengembalikan fungsinya maka harus dilakukan perawatan rekonstruksi tulang alveolar. Baku emas dalam perawataan ini ialah menggunakan autologous bone grafting. Namun, perawatan ini masih memiliki kekurangan sehingga dikembangkan perawatan yang baru dengan teknik rekayasa jaringan dengan sel punca mesenkim. Salah satu sumber sel punca mesenkim yaitu berasal dari jaringan pulpa gigi yaitu sel punca pulpa gigi permanen atau dental pulp stem cells (DPSCs) dan sel punca pulpa gigi sulung atau stem cells from human deciduous teeth (SHED). Kemampuan osteogenik dari sel punca merupakan salah satu faktor pertimbangan untuk pemakaian sel dalam rekayasa jaringan rekonstruksi tulang. Sementara kemampuan osteogenik dari SHED dan DPSCs CLP belum diketahui. Tujuan: Mengetahui potensi kemampuan dan perbandingan potensi osteogenik dari sel punca gigi permanen dan sulung pasien celah bibir dan palatum dengan melihat ekspresi gen Alkaline phosphatase (ALP) dan Collagen Type I Alpha 1 (COL1A1). Metode: Sampel RNA yang diperoleh dari ekstraksi RNA sel jaringan pulpa gigi sulung dan permanen pasien celah bibir dan palatum diuji dengan Real-Time Polymerase Chain Reaction (RT-PCR) menggunakan primers Alkaline Phosphatase (ALP), Collagen Type-I (COL1A1) dan Glyceraldehyde 3-Phosphate Dehydrogenase (GAPDH) sebagai housekeeping gene. Hasil: Ekspresi relatif gen ALP pada sel punca pulpa gigi sulung pasien celah bibir dan palatum mengalami penurunan dibandingkan dengan sel punca gigi permanen pasien celah bibir dan palatum. Sementara untuk ekspresi gen COL1A1 pada sel punca pulpa gigi sulung pasien celah bibir dan palatum tidak memiliki perbedaan dibandingkan dengan sel punca gigi permanen pasien celah bibir dan palatum. Kesimpulan: Sel punca pulpa gigi sulung dan permanen pasien celah bibir dan palatum memiliki potensi kemampuan osteogenik dikarenakan keduanya mengekspresikan gen marker osteogenik seperti ALP dan COL1A1. ......Background: Cleft lip and palate (CLP) is a multifactorial congenital disorder that results in patients having soft and hard tissue defects in the lips and palate. Patients with cleft lip and palate commonly suffer from aesthetic and stomatognathic function disorders. Therefore, to restore its function, alveolar bone reconstruction treatment must be done. The gold standard in this treatment is to perform autologous bone grafting. However, as autologous bone grafting still has associated shortcomings, new treatments using tissue engineering techniques with mesenchymal stem cells are being developed. One of the mesenchymal stem cells sources that can be used is derived from dental pulp tissue, namely permanent dental pulp stem cells (DPSCs) and primary dental pulp stem cells or stem cells from human deciduous teeth (SHED). Osteogenic ability of the stem cells is one of the factors considered for the use of cells in tissue engineering bone reconstruction. Osteogenic ability of SHED and DPSCs hasn’t been fully explored. Objective: To determine the potential ability and to compare osteogenic potential of DPSCs and SHED from cleft lip and palate patients by looking at the expression of the Alkaline Phosphatase (ALP) and Collagen Type I Alpha 1 (COL1A1) genes. Methods: RNA samples obtained from RNA cells extraction in deciduous and permanent dental pulp tissue of patients with cleft lip and palate were tested with Real-Time Polymerase Chain Reaction (RT-PCR) using Alkaline Phosphatase (ALP) primers, Collagen Type I Alpha 1 (COL1A1) primers and Glyceraldehyde 3-Phosphate Dehydrogenase (GAPDH) primers as housekeeping gene. Results: The relative expression of ALP genes in SHED from CLP patients decreased compared to DPSCs from patients with CLP. As for the expression of the COL1A1 gene, there was no difference in expression between SHED from patients with cleft lip and palate and DPSCs in patients with cleft lip and palate. Conclusion: SHED and DPSCs CLP has osteogenic abilities.

Abstrak :
Latar Belakang: L-arginin merupakan asam amino semiesensial yang produksinya tidak mencukupi kebutuhan dalam kondisi stres oksidatif akibat inflamasi. L-arginin adalah satu-satunya substrat bagi enzim nitric oxide synthase (NOS) yang memproduksi nitric oxide (NO) yang dapat mengaktivasi focal adhesion kinase (FAK) pathwaydan memicu terjadinya proses migrasi sel. Tujuan: Mengetahui potensi media kultur asam amino L-arginin terhadap laju kecepatan migrasi hDPSCs. Metode: Evaluasi media kultur asam amino L-arginin konsentrasi 300, 400, 500 ¼mol/L, serta DMEM sebagai kontrol terhadap laju kecepatan migrasi hDPSCs menggunakan uji scratch assay menggunakan uji scratch assay yang dihitung dengan rumus laju kecepatan migrasi setelah 24 jam. Analisis statistic menggunakan Paired T-Test dan Oneway ANOVA dengan post hoc LSD. Hasil: Terdapat perbedaan bermakna potensi L-arginin 500 μmol/L dibandingkan konsentrasi 300 dan 400 μmol/L, serta kontrol. Kesimpulan: Media kultur asam amino L-arginin 500 ¼mol/L memiliki potensi laju kecepatan migrasi yang lebih baik dibandingkan konsetrasi 300, 400 ¼mol/L dan kontrol. ...... Background: L-arginine is semiessential amino acid which the production is insufficient under oxidative stress due to inflammation. L-arginine is the only substrate of nitric oxide synthase (NOS) enzyme that produces nitric oxide (NO) which activates focal adhesion kinase (FAK) pathway to stimulate cell migration. Objective: To understand potential of L-arginine amino acid culture media towards speed rate of hDPSCs migration. Methods: Evaluation of 300, 400, 500 ¼mol/L of L-arginin amino acid culture media and DMEM as control towars speed rate of hDPSCs migration using scratch assay and calculation of migration speed rate after 24 hours. Statistical analysis using Paired T-Test and Oneway ANOVA with post hoc LSD. Results: Significant result was shown between 500 ¼mol/L of L-arginin amino acid culture media compared with 300 and 400 ¼mol/L concentration and control towards migration speed rate after 24 hours. Conclusion: 500 ¼mol/L of L-arginin amino acid culture media has a better migration rate compared with lower concentrations and control.