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"Latar belakang: Cedera saraf perifer merupakan komplikasi trauma ekstremitas pada 3-10 pasien yang menyebabkan kelainan fungsi normal saraf. Terapi sel punca mesenkimal MSC telah banyak dikembangkan untuk regenerasi sel dan jaringan. Conditioned medium CM yang berasal dari tali pusat MSC-TP manusia dalam regenerasi saraf perifer belum banyak diketahui. Penelitian ini bertujuan untuk membandingkan perbaikan fungsi dan struktur saraf perifer.Metode: Penelitian ini merupakan penelitian eksperimental menggunakan 36 ekor tikus putih Rattus norvegicus berumur 2-3 bulan dengan berat badan berkisar 250-300 g. Penelitian dilakukan di laboratorium RSCM-FKUI dan Pusat Penelitian dan Pengembangan selama 3 tahun. Hewan coba dibagi menjadi 3 kelompok, yaitu kelompok kontrol atau sham SH , terapi standar ST , dan perlakuan conditioned medium MSC-TP CM . Penelitian dibagi menjadi dua jangka waktu, yaitu jangka pendek 7 hari pasca operasi HPO dan jangka panjang 70 HPO . Pemeriksaan yang dilakukan adalah analisis berjalan, elektrofisiologi dan imunohistokimia.Hasil: Hasil pemeriksaan fungsi motorik SFI, TFI, PFI, Q1-Q4 dan TOA , kelompok CM menunjukkan kesembuhan yang lebih cepat dibanding kelompok ST. Hasil gambaran elektrofisiologi, kelompok CM memiliki kecepatan konduksi saraf NCV lebih baik dibandingkan kelompok ST. Berdasarkan gambaran histologis, pewarnaan HE menunjukkan jumlah sel saraf yang lebih banyak pada kelompok CM dibanding kelompok ST pada hari ke-7 HPO dan 70 HPO. Pewarnaan TB menunjukkan diameter selubung mielin yang lebih tebal pada kelompok CM dibandingkan kelompok ST pada hari ke-7 HPO dan 70 HPO. Marker CD34 menunjukkan jumlah pembuluh darah memiliki hasil pada kelompok CM yang mendekati kelompok SH pada hari ke-7 HPO dan 70 HPO. Marker S100 menunjukkan persentase yang lebih banyak pada kelompok CM dibanding kelompok ST pada hari ke-7 HPO dan 70 HPO.Kesimpulan: CM MSC-TP mampu memberikan pengaruh terhadap perbaikan struktur dan fungsi saraf perifer pascacedera saraf pada kelompok CM hari ke-7 HPO.

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Background Peripheral nerve injury is a complication of extremities trauma in 3 10 of patients causing the dysfunction of nerve. Mesenchymal stem cell conditioned medium MSC CM is used as therapy to regenerate cells and tissues. However, the ability of human umbilical cord derived mesenchymal stem cell conditioned medium HU MSC CM in regenerating peripheral nerves has not been known. This research aimed to compare the functional and structural repairs of peripheral nerve.

Method This study is an experimental research using 36 rats of Sprague Dawley Rattus norvegicus strain aged 2 3 months with body weight ranging from 250 to 300 grams. The research was conducted in various laboratories at RSCM FKUI and the Center for Health Research and Development for three years. The experimental animals were divided into 3 groups, namely the control group SH , the standard therapy treatment group ST , and the conditioned medium treatment group CM . The research was divided into two stages consisting of a short term research of 7 days of post surgery PS and a long term research 70 PS . The examinations performed were in the form of motor function for the walking analysis, electrophysiology, and immunohistochemistry.

Result Based on the examination of motor function SFI, TFI, PFI, Q1 Q4, and TOA , the CM group showed faster recovery compared to the ST group. Based on the electrophysiological images, the CM group was able to have a better nerve conduction velocity NCV compared to the ST group. Based on the histological images, HE staining showed a higher amount of all nerve cells in the CM group compared to the amount in the ST group on the 7th day of PS and 70th day of PS. TB staining showed a thicker myelin sheath diameter in the CM group than that in the ST group on the 7th day of PS and 70th day of PS. CD34 marker showed that the number of blood vessels of the CM group was close to that of the SH group on the 7th day of PS and 70th day of PS. S100 marker had a higher percentage in the CM group compared to the ST group on the 7th day of PS and 70th day of PS.

Conclusion HU MSC CM is able to affect the functional and structural repairs of the peripheral nerve after nerve injury in the CM group on the 7th day of PS."

"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"

"Latar Belakang: Uji tube formation merupakan uji paling luas yang digunakan sebagai uji vaskulogenesis/ angiogenesis secara in vitro. Sel punca mesenkimal atau mesenchymal stem cell MSC merupakan sel punca dewasa yang multipoten. Efek parakrinnya terhadap neovaskularisasi sudah banyak diketahui. Secara umum MSC diketahui tidak mengekspresikan penanda permukaan hematopoetik CD34 namun ada pendapat yang menyatakan bahwa MSC secara in vivo mengekspresikan CD34 dan kehilangan ekspresinya saat dikultur secara in vitro. MSC asal lemak dianggap masih memiliki ekspresi CD34 pada kultur in vitro pada pasase awal oleh beberapa ahli. MSC yang paling banyak digunakan dalam uji tube formation adalah BM-MSC padahal ASC juga berpotensi bagi terapi dan rekayasa sel punca. Hingga saat ini potensi vaskulogenesis antara ASC dan BM-MSC masih belum jelas mana yang lebih baik dan apakah ekspresi CD34 mempengaruhi hal ini. Pada penelitian ini kami ingin membandingkan potensi vaskulogenesis antara MSC asal lipoaspirat dengan MSC asal sumsum tulang melalui uji tube formation dan ekspresi CD34. Hasil: Pengukuran kualitas vaskulogenesis menunjukkan bahwa rerata panjang tube lebih tinggi pada BM-MSC, rerata jumlah loop lebih banyak pada BM-MSC dan rerata jumlah titik percabangan lebih banyak pada BM-MSC. Tidak ditemukan kadar CD34 yang tinggi pada ASC. Kesimpulan: BM-MSC memiliki kemampuan lebih baik dalam membentuk tube formation dibandingkan dengan ASC. Tidak ditemukan hubungan antara kadar CD34 dengan kemampuan vaskulogenesis MSC.

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Objective: Test tube formation is the most widely used method as an in vitro vasculogenesis test. Mesenchymal stem cells MSC is a multipotent adult cells known not expressing CD34 just like endothelial progenitor cells EPC that play a role in vasculogenesis. Adipose derived stem cells MSCs ASC is considered to still express CD34 2 in cultures. Bone Marrow BM MSCs is most widely used MSCs in vasculogensis research. ASC has great potential for stem cell therapy and engineering. The potential of vasculogenesis between ASC and BM MSC remains unclear which one is better and whether CD34 expression affects this. In this study we wanted to compare the potential of vasculogenesis between MSC of lipoaspiric origin and MSC from bone marrow through tube formation test and CD34 expression. Tube formation assay is the most widely used method as an in vitro vasculogenesis test. Mesenchymal stem cells MSCs are multipotent adult cells. known not to express CD34 surface marker which is expressed by haemapoietic stem cells, but according to some experts bone marrow mesenchymal stem cells BM MSCs express CD34 in vivo and lose its expression when they are cultured in vitro, while adipose derived stem cells ASCs still have CD34 expression in the early passages when cultured in vitro. BM MSCs are the most widely used MSC, but ASCs are also used in stem cell therapy and tissue engineering for angiogenesis purposes. Until now the potential of vasculogenesis between ASCs and BM MSCs is still unclear. Expression of CD34 is also unknown whether effecting the quality of tube formation. In this study we wanted to compare the potential of vasculogenesis between ASC and BM MSCs through tube formation test and CD34 expression.

Results: Measurements of vasculogenesis quality showed higher tube length, number of loops and mean number of branch points on BM MSC. Both BM MSCs and ASCs showed low CD34 levels.

Conclusion: BM MSCs showed better tube formation ability compared with ASCs. No association was found between CD34 levels and MSC vasculogenesis capability. "

"Latar belakang: Celah bibir dan palatum (CLP) adalah kegagalan fusi prosesus frontonasal dan maksilaris yang menghasilkan celah yang meluas ke bibir, alveolus, dasar hidung, dan palatum keras maupun lunak. Diperlukan perawatan melalui teknik rekayasa jaringan dengan menggunakan sel stromal mesenkim yang dapat ditemukan pada dental pulp stromal cells (DPSC). Kemampuan osteogenik DPSC dapat dilihat melalui deteksi marker osteogenik seperti osteopontin (OPN). Osteopontin merupakan salah satu marker utama diferensiasi osteogenik yang diproduksi oleh osteoblas dalam proses pembentukan dan mineralisasi tulang. Pada pasien CLP diketahui perbedaan ekspresi gen yang dapat memengaruhi sintesis matriks ekstraseluler. Penelitian ini dilakukan untuk mengetahui kemampuan diferensiasi osteogenik melalui ekspresi marker osteopontin saat diferensiasi osteoblas pada pasien celah bibir dan palatum. Tujuan: Membandingkan kemampuan diferensiasi osteogenik sel stromal pulpa gigi subjek normal dengan sel stromal pulpa gigi pasien celah bibir dan palatum melalui ekspresi gen osteopontin. Metode: Sampel RNA yang diperoleh dari kultur sel pulpa gigi subjek normal dan pasien celah bibir dan palatum diuji dengan Real-Time Polymerase Chain Reaction (RT-PCR) dengan primer osteopontin (OPN) dan 18S sebagai housekeeping gene. Hasil: Tidak terdapat perbedaan antara ekspresi relatif gen OPN sel stromal pulpa gigi subjek normal dan pasien celah bibir dan palatum. Kesimpulan: Kemampuan diferensiasi osteogenik sel stromal pulpa gigi pada pasien celah bibir dan palatum ekuivalen dengan sel stromal pulpa gigi pada subjek normal.

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Background: Cleft lip and palate (CLP) occurs due to the failure of fusion of the frontal and maxillary process that results in a cleft that extends to the lip, alveoli, nose floor, and hard and soft palate. One of the potentially alternative treatment for CLP cases is tissue engineering technique using Mesenchymal Stromal Cell (MSC). MSC can be found in dental pulp stromal cells (DPSC). Osteogenic ability can be seen through the detection of osteogenic markers such as osteopontin (OPN). Osteopontin is one of the main markers of osteogenic differentiation produced by osteoblast in the process of bone formation and mineralization. Osteopontin is expressed by preosteoblasts in early bone formation and mature osteoblasts at bone remodelling sites. Osteopontin expression as one of osteogenic markers in cleft lip and palate patients is unknown. This study was conducted to determine the ability of osteogenic differentiation through the expression of osteopontin in cleft lip and palate patients. Objective: To compare osteogenic differentiation ability of mesenchymal stromal cells in cleft lip and palate patients and normal subject through the expression of osteogenic marker osteopontin. Methods: RNA sample that was obtained through RNA extraction from dental pulp stromal cells of cleft and lip palate patients and normal subjects were tested with Real-Time Polymerase Chain Reaction (RT-PCR) using osteopontin and 18S as housekeeping gene. Results: There was no difference between the relative expression of OPN gene in DPSC from normal subject and cleft lip and palate patients. Conclusion: Osteogenic differentiation ability of dental pulp stromal cells from cleft lip and palate patients is equivalent with dental pulp stromal cells from normal subjects."