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"ABSTRACTThis study has been conducted to obtain possible correlation between Calcium concentration in the enamel of Incisive deciduous teeth of 6 to S years children in the Elementary school and tee caries experience of the same teeth. The hypothesis is teat the caries experience is in parallel correlation with the Calcium concentration of, the affected teeth. The cross sectional study involves 53 selected children among 327 children examinee. Factor which influences the concentration of Calcium in tr7e enamel is the intake of Calcium of samples when they were still babies, whereas factor which influences caries is the plaque. It is found that there is no correlation between higher Calcium concentration and less caries experience (p>0.005). There is no significant difference in the concentration of Calcium between negative and positive caries children (p >. 0.05). No significant difference is also found in the intakes Calcium of samples when they were still babies correlated with the concentration of Calcium in the enamel of samples (p > 0.05). There is no significant correlation between the caries experience and the plaque level 0.05). The hypothesis is not supported by the data obtained. Higher Calcium concentration in enamel is not related to less caries experience. Longitudinal study which involves higher sample number is needed to observe the interaction of one variable to another to achieve better result of the similar study."

"Latar Belakang : DPSC dan SHED merupakan sumber sel stromal yang dapat digunakan untuk rekayasa jaringan sebagai alternatif perawatan pasien dengan CLP. Penelitian terdahulu menunjukkan ekspresi gen Homeobox pada DPSC pasien dengan CLP dibandingkan subjek normal. Gen Homeobox merupakan sekelompok gen yang mengkodekan serangkaian domain protein yang berperan dalam proses awal perkembangan dan diferensiasi sel saat embriogenesis. Dalam kelompok homeobox ini, terdapat gen SHOX yang berperan dalam pembentukan kerangka tulang pada tahap embriogenesis. Penelitian ini dilakukan untuk memvalidasi perbedaan ekspresi gen pada kelompok sampel DPSC dan SHED subjek normal dan pasien CLP. Tujuan : Melakukan evaluasi karakteristik sel pada sampel DPSC subjek normal dengan pasien CLP; DPSC dengan SHED pasien CLP. Metode : Menggunakan template RNA dari 3 kelompok sampel yaitu DPSC subjek normal, DPSC pasien CLP, dan SHED pasien CLP. Lalu, sintesis cDNA dan dilakukan metode RT-qPCR untuk melihat ekspresi gen SHOX dari setiap kelompok sampel. Hasil : Tidak terdapat perbedaan ekspresi gen SHOX pada perbandingan kelompok sampel DPSC normal dengan pasien CLP, dan kelompok DPSC CLP dengan SHED CLP. Kesimpulan : DPSC dan SHED subjek normal dan pasien CLP memiliki karakteristik gen SHOX yang sama.

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Background : DPSC and SHED are the sources for tissue engineering as an alternative treatment for patients with CLP. Previous studies showing expression of homeobox genes in DPSC of normal compared to CLP patients. Homeobox genes encode a series of protein domains that is involved in the process of development and cell differentiation. There is a SHOX gene involved in the bone skeleton formation during embryogenesis. This study was conducted to validate the differences in gene expression between the sample groups of DPSC and SHED of normal and CLP subjects. Objective : To evaluate the cell characteristics in sample groups of DPSC in normal and CLP subjects; DPSC and SHED in CLP subjects. Methods : Using RNA template of 3 sample groups, namely DPSC of normal subjects, DPSC of CLP subjects. cDNA was synthesized and the RT-qPCR method was used to see the SHOX gene expression of each group. Result : There was no differences in SHOX gene expression in the comparison of DPSC normal with CLP patients, and the DPSC and SHED in subjects with CLP. Conclusion : DPSC and SHED in normal subjects and CLP patients have the same characteristics of SHOX gene."

"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.

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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."

"Latar Belakang: Subjek celah bibir dan palatum membutuhkan perawatan rekonstruksi tulang berbasis rekayasa jaringan dengan menggunakan sel stromal mesenkim. Sel stromal mesenkim merupakan sel yang banyak digunakan untuk regenerasi tulang karena mempunyai kemampuan proliferasi tinggi. Sel tersebut dapat berasal dari pulpa gigi sulung (SHED) danpulpa gigi permanen (DPSCs) yang dapat berdiferensiasi menjadi osteoblas. Pada penelitiansebelumnya telah ditemukan beberapa karakteristik DPSCs dan SHED pada subjek celah bibir dan palatum, namun kemampuan diferensiasi dari sel stromal pulpa subjek celah bibir dan palatum belum diketahui. Tujuan: Mengevaluasi kemampuan diferensiasi osteogenik dari sel stromal pulpa gigi permanen dan sulung pada subjek celah bibir dan palatum melaluiekspresi gen Collagen Type I Alpha I (COL1A1). Metode : Sampel RNA yang diperoleh dari kultur RNA DPSCs dan SHED subjek celah bibir dan palatum, dengan Real-Time Polymerase Chain Reaction (RT-PCR) menggunakan primers Collagen Type I Alpha I (COL1A1), serta 18S sebagai housekeeping gene. Hasil : Tidak terdapat perbedaan ekspresi relatif gen COL1A1 antara sel stromal pulpa gigi permanen dan sel stromal pulpa gigi sulung pada subjek celah bibir dan palatum. Kesimpulan : SHED memiliki kemampuan diferensiasi osteogenik yang sama dengan DPSCs karena keduanya dapat mengekspresikan gen marker osteogenik COL1A1.

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Background: Cleft lip and palate subject need bone reconstruction based tissue engineering treatment with mesenchymal stromal cells (MSC). One of the most mesenchymal stromal cells that can be used is derived from dental pulp tissues, such as primary tooth pulp or stem cells from human deciduous teeth (SHED) and dental pulp stem cells (DPSCs) which can differentiate into osteoblasts. In previous studies, several characteristics of DPSCs and SHED of the cleft lip and palate subjects have been found. However, osteogenic differentiation ability of dental pulp stromal cells from cleft lip and palate subject is unknown.

Objective: To determine the osteogenic differentiation ability of DPSCs and SHED of cleft lip and palate subjects through the expression of the Collagen Type I Alpha I (COL1A1) gene.

Methods: RNA samples obtained from the culture of DPSCs and SHED of lip and palate cleft subjects, with Real-Time Polymerase Chain Reaction (RT-PCR) using primers Collagen Type I Alpha I (COL1A1) and 18S as a housekeeping gene.

Results: There was no difference in the relative expression of COL1A1 gene between DPSCs and SHED of CLP subjects.

Conclusion: SHED has the same osteogenic differentiation ability as DPSCs because they can express osteogenic marker genes COL1A1."

"Latar Belakang: Celah bibir dan palatum merupakan salah satu kelainan bawaan yang menyebabkan defek jaringan keras sehingga dikembangkan perawatan rekonstruksi tulang berbasis teknik rekayasa jaringan sebagai alternatif perawatan. Sumber sel stromal mesenkim dapat diperoleh dari pulpa gigi sulung dan gigi permanen. Kemampuan diferensiasi osteogenik sel stromal pulpa gigi sulung dan gigi permanen sudah banyak dilaporkan. Pada pasien celah bibir dan palatum, terdapat gen-gen yang diekspresikan berbeda dan kemampuan diferensiasi osteogenik sel stromal pulpa gigi sulung dan gigi permanen pasien celah bibir dan palatum belum diketahui. Tujuan: Mengevaluasi perbandingan kemampuan diferensiasi osteogenik sel stromal pulpa gigi sulung dan gigi permanen pasien celah bibir dan palatum melalui deposisi kalsium. Metode: Sel stromal pulpa gigi sulung dan gigi permanen pasien celah bibir dan palatum dikultur menggunakan medium osteogenik selama 21 hari kemudian dilakukan pewarnaan Alizarin Red dan kuantifikasi terhadap deposisi kalsium. Hasil: Sel stromal pulpa gigi sulung dan gigi permanen yang dikultur menggunakan medium osteogenik menunjukkan adanya deposisi kalsium yang tinggi. Sel stromal pulpa gigi sulung dan gigi permanen tidak menunjukkan perbedaan nilai rerata absorbansi, intensitas pewarnaan, dan area pewarnaan yang bermakna secara statistik (p ≥ 0,05). Kesimpulan: Sel stromal pulpa gigi sulung pasien celah bibir dan palatum memiliki kemampuan diferensiasi osteogenik yang ekuivalen dengan sel stromal pulpa gigi permanen pasien celah bibir dan palatum.

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Background: Cleft lip and palate is one of the most common congenital anomalies resulting in hard tissue defects therefore tissue engineering is currently developed as an alternative treatment. The source of mesenchymal stromal cells can be obtained from human exfoliated deciduous teeth (SHED) and dental pulp (DPSCs). Osteogenic differentiation abilities of SHED and DPSCs have been widely studied. In cleft lip and palate patients, there are several differentially expressed genes and the osteogenic differentiation abilities of SHED and DPSCs in cleft lip and palate patients have not yet been known. Purpose: To compare the osteogenic differentiation abilities of SHED and DPSCs in cleft lip and palate patients by calcium deposition. Methods: SHED and DPSCs isolated from cleft lip and palate patients were cultured using osteogenic medium for 21 days then added Alizarin Red staining and the calcium deposition were quantified. Result: Both SHED and DPSCs that cultured in osteogenic medium demonstrated high calcium deposition. SHED and DPSCs did not show any statistically significant differences in the average absorbance values, staining intensity, and staining areas (p ≥ 0,05). Conclusion: SHED and DPSCs in cleft lip and palate patients have equivalent ability of osteogenic differentiation by calcium deposition."