Hasil Pencarian  ::  Simpan CSV :: Kembali

"Deteksi Infeksi Submikroskopis Necator americanus, Ancylostoma duodenale, dan Ascaris lumbricoides dari Sampel Feses di Nangapanda, Ende, Menggunakan Real-Time Polymerase Chain Reaction. Infeksi dari Soil-Transmitted Helminthes (STH) (N. americanus, A. duodenale (Hookworm), dan A. lumbricoides) dapat menyebabkan anemia, kekurangan zat besi, bahkan malnutrisi. Pemeriksaan infeksi STH dapat dilakukan menggunakan mikroskop, tetapi metode tersebut masih kurang sensitif. Penelitian bertujuan mendeteksi dan mengetahui persentase infeksi submikroskopis STH dari sampel feses anak (usia 5-18 tahun) di Nangapanda, Ende menggunakan metode real-time polymerase chain reaction (PCR). Sampel feses dikoleksi sebanyak dua kali, yaitu sebelum dan sesudah pemberian albendazole 400 mg. Total sampel yang diperoleh adalah 242 tetapi hanya 45 sampel yang negatif secara mikroskopis yang diuji dengan real-time PCR. DNA sampel diisolasi dan diamplifikasi menggunakan primer dari daerah internal transcribed spacer (ITS-1 dan ITS-2) rDNA. Deteksi dengan real-time PCR menghasilkan kurva amplifikasi pada fluorophore VIC, FAM, dan Texas Red. Sebanyak tiga sampel (6,7%) pada pre treatment termasuk low load of DNA (N. americanus and A. lumbricoides) (Ct > 35), empat sampel (9,1%) termasuk low load of DNA untuk N. americanus saja (Ct > 35), dan lima sampel (11,4%) termasuk moderate load of DNA untuk A. lumbricoides saja (30 < Ct < 35) pada post treatment. Hasil penelitian menunjukkan bahwa real-time PCR dapat mendeteksi infeksi submikroskopis dari Hookworm dan A. lumbricoides.

---

Soil-transmitted helminth (STH) infections (Necator americanus (hookworm), Ancylostoma duodenale (hookworm), and Ascaris lumbricoides) can lead to anemia, malnutrition, and iron deficiency. Traditionally, STH infections have been diagnosed using microscopy to detect eggs in human fecal samples. However, there are several limitations of this method. The aim of this research was to detect the percentage of submicroscopic STH infections from human fecal samples (children, 5?18 years old) in Nangapanda, Ende, using the real-time polymerase chain reaction (PCR) method. The fecal samples were collected in two time periods, which were before and after treatment, using 400 mg of Albendazole. There were 242 samples in total, but only 45 negative samples from microscopic detection were tested with real-time PCR. The DNA samples were isolated and amplified wih primers of internal transcribed spacer (ITS-1 and ITS-2) region of rDNA. The detection of samples with real-time PCR generated an amplification curve in VIC, FAM, and Texas Red fluorophore. Three samples (6.7%) in pre-treatment were low load of DNA (N. americanus and A. lumbricoides) (Ct > 35). Four samples (9.1%) were low load of DNA (N. americanus) (Ct > 35) in post-treatment. Five samples (11.4%) were moderate load of DNA (A. lumbricoides) (30 < Ct < 35) in post-treatment. real-time PCR could detect submicroscopic infections from specific species of hookworm and A. lumbricoides."

"Deteksi Infeksi Submikroskopis Necator americanus, Ancylostoma duodenale, dan Ascaris lumbricoides dari Sampel Feses di Nangapanda, Ende, Menggunakan Real-Time Polymerase Chain Reaction. Infeksi dari Soil-Transmitted Helminthes (STH) (N. americanus, A. duodenale (Hookworm), dan A. lumbricoides) dapat menyebabkan anemia, kekurangan zat besi, bahkan malnutrisi. Pemeriksaan infeksi STH dapat dilakukan menggunakan mikroskop, tetapi metode tersebut masih kurang sensitif. Penelitian bertujuan mendeteksi dan mengetahui persentase infeksi submikroskopis STH dari sampel feses anak (usia 5-18 tahun) di Nangapanda, Ende menggunakan metode real-time polymerase chain reaction (PCR). Sampel feses dikoleksi sebanyak dua kali, yaitu sebelum dan sesudah pemberian albendazole 400 mg. Total sampel yang diperoleh adalah 242 tetapi hanya 45 sampel yang negatif secara mikroskopis yang diuji dengan real-time PCR. DNA sampel diisolasi dan diamplifikasi menggunakan primer dari daerah internal transcribed spacer (ITS-1 dan ITS-2) rDNA. Deteksi dengan real-time PCR menghasilkan kurva amplifikasi pada fluorophore VIC, FAM, dan Texas Red. Sebanyak tiga sampel (6,7%) pada pre treatment termasuk low load of DNA (N. americanus and A. lumbricoides) (Ct > 35), empat sampel (9,1%) termasuk low load of DNA untuk N. americanus saja (Ct > 35), dan lima sampel (11,4%) termasuk moderate load of DNA untuk A. lumbricoides saja (30 < Ct < 35) pada post treatment. Hasil penelitian menunjukkan bahwa real-time PCR dapat mendeteksi infeksi submikroskopis dari Hookworm dan A. lumbricoides.

---

Soil-transmitted helminth (STH) infections (Necator americanus (hookworm), Ancylostoma duodenale (hookworm), and Ascaris lumbricoides) can lead to anemia, malnutrition, and iron deficiency. Traditionally, STH infections have been diagnosed using microscopy to detect eggs in human fecal samples. However, there are several limitations of this method. The aim of this research was to detect the percentage of submicroscopic STH infections from human fecal samples (children, 5?18 years old) in Nangapanda, Ende, using the real-time polymerase chain reaction (PCR) method. The fecal samples were collected in two time periods, which were before and after treatment, using 400 mg of Albendazole. There were 242 samples in total, but only 45 negative samples from microscopic detection were tested with real-time PCR. The DNA samples were isolated and amplified wih primers of internal transcribed spacer (ITS-1 and ITS-2) region of rDNA. The detection of samples with real-time PCR generated an amplification curve in VIC, FAM, and Texas Red fluorophore. Three samples (6.7%) in pre-treatment were low load of DNA (N. americanus and A. lumbricoides) (Ct > 35). Four samples (9.1%) were low load of DNA (N. americanus) (Ct > 35) in post-treatment. Five samples (11.4%) were moderate load of DNA (A. lumbricoides) (30 < Ct < 35) in post-treatment. real-time PCR could detect submicroscopic infections from specific species of hookworm and A. lumbricoides."

"ABSTRAK Latar belakang : Cytomegalovirus (CMV) merupakan salah satu infeksi oportunistikpada pasien dengan sindrom immunodefisiensi (AIDS). Gejala klinis dan CT scantidak dapat menegakkan diagnosa definitif ensefalitis CMV. Oleh karena itudiperlukan uji alternatif untuk menegakkan diagnosis infeksi CMV pada pasien HIVdengan infeksi otak. Salah satu uji yang sensitif dan spesifik adalah Real TimePolymerase Chain Reaction (rPCR).Tujuan : Mendapatkan uji deteksi molekular CMV pada pasien HIV dengantersangka infeksi otak.Metode : Penelitian dilakukan dalam 3 tahap. Tahap 1 adalah optimasi konsentrasiprimer, probe, suhu annealing, volume elusi ekstraksi DNA, dan volume cetakan.Tahap 2 adalah uji spesifisitas (reaksi silang) dan uji sensitivitas (ambang batasdeteksi DNA) rPCR dan tahap 3 adalah penerapan uji rPCR yang sudah dioptimasiterhadap sampel plasma, urin, dan LCS.Hasil : Kondisi optimal uji rPCR telah diperoleh dengan konsentrasi primer danprobe 0,1 μM, dengan kondisi suhu reaksi rPCR: aktivasi enzim pada 950C selama 3menit; 45 siklus pada 950C selama 15 detik (denaturasi) dan 560C selama 1 menit(annealing dan ekstensi). Volume elusi ekstraksi DNA yang optimal untuk ketigajenis sampel (LCS, plasma dan urin) adalah 40 μL, dan volume cetakan rPCR untukLCS, plasma, dan urin, masing-masing adalah 5, 4, dan 3 μL. Uji rPCR mampumendeteksi DNA pada 50.000 jumlah kopi/mL dan tidak bereaksi silang denganStaphylococcus aureus, Staphylococcus epidermidis, Staphylococcus saprophyticus,Escherichia coli, Klebsiella pneumoniae, Pseudomonas aeruginosa, Mycobacteriumtuberculosis, Candida spp, Toxoplasma gondii, EBV,HSV,dan VZV. Penerapan ujirPCR pada sampel klinis memberikan hasil negatif pada semua sampel LCS, 72,22%positif pada sampel plasma, dan 72,22% positif pada sampel urin.Kesimpulan: Telah dilakukan optimasi uji rPCR dengan minimal deteksi DNACMV 50.000 jumlah kopi/mL dan tidak bereaksi silang dengan mikroorganisme yangberpotensi menyebabkan positif palsu (false positive).ABSTRACT Background: Cytomegalovirus (CMV) is one of opportunistic infections in patientswith Aquired Immunodeficiency Syndrome (AIDS). Clinical manifestations are nottypical, and CT scans can not define encephalitis CMV specifically. Therefore, it isimportant to apply an alternative assay for sensitive and specific detection of CMVinfection in HIV patients with suspected central nervous system (CNS) infections.One of the assays is real time polymerase chain reaction (rPCR).Objective: To obtain a molecular assay for detection of CMV in HIV patients withsuspect CNS infections.Methods: This study was conducted in three phases. The first is optimization ofconcentrations of primers, probe, annealing temperature, final elution of DNAextraction, and volume of PCR template. The second is determinations of sensitivity(minimal detection of DNA) and specificity (cross-reaction) of the optimized rPCR,and the third is application of the rPCR for clinical samples of plasma, urine, andliquor cerebrospinal (LCS).Results: The rPCR reaction showed optimal concentrations of primers and probe at0.1 μM, with thermal cycler: 950C for 3 min (enzyme activation), followed by 45cycles of 950C for 15 sec (denaturation) and 560C for 1 min (annealing andextension). Final elution of DNA extraction was 40 μL and volume of PCR templatesfor urine, plasma, and LCS was 3, 4, and 5 μL, respectively. The rPCR had minimaldetection of DNA at 50,000 copies/mL and was not cross-reacted withStaphylococcus aureus, Staphylococcus epidermidis, Staphylococcus saprophyticus,Escherichia coli, Klebsiella pneumoniae, Pseudomonas aeruginosa, Mycobacteriumtuberculosis, Candida spp, Toxoplasma gondii, Epstein-Bar Virus (EBV), HerpesSimplex Virus (HSV) and Varicella Zoster Virus (VZV). Application of rPCR forclinical samples showed that the rPCR yielded 72.22% positive for plasma or urine,and negative for all LCS samples.Conclusion: The rPCR has been optimized in this study with minimal DNA detectionat 50,000 copies/mL and was not cross-reacted with other microorganisms that arepotential to cause false positive results.;Background: Cytomegalovirus (CMV) is one of opportunistic infections in patientswith Aquired Immunodeficiency Syndrome (AIDS). Clinical manifestations are nottypical, and CT scans can not define encephalitis CMV specifically. Therefore, it isimportant to apply an alternative assay for sensitive and specific detection of CMVinfection in HIV patients with suspected central nervous system (CNS) infections.One of the assays is real time polymerase chain reaction (rPCR).Objective: To obtain a molecular assay for detection of CMV in HIV patients withsuspect CNS infections.Methods: This study was conducted in three phases. The first is optimization ofconcentrations of primers, probe, annealing temperature, final elution of DNAextraction, and volume of PCR template. The second is determinations of sensitivity(minimal detection of DNA) and specificity (cross-reaction) of the optimized rPCR,and the third is application of the rPCR for clinical samples of plasma, urine, andliquor cerebrospinal (LCS).Results: The rPCR reaction showed optimal concentrations of primers and probe at0.1 μM, with thermal cycler: 950C for 3 min (enzyme activation), followed by 45cycles of 950C for 15 sec (denaturation) and 560C for 1 min (annealing andextension). Final elution of DNA extraction was 40 μL and volume of PCR templatesfor urine, plasma, and LCS was 3, 4, and 5 μL, respectively. The rPCR had minimaldetection of DNA at 50,000 copies/mL and was not cross-reacted withStaphylococcus aureus, Staphylococcus epidermidis, Staphylococcus saprophyticus,Escherichia coli, Klebsiella pneumoniae, Pseudomonas aeruginosa, Mycobacteriumtuberculosis, Candida spp, Toxoplasma gondii, Epstein-Bar Virus (EBV), HerpesSimplex Virus (HSV) and Varicella Zoster Virus (VZV). Application of rPCR forclinical samples showed that the rPCR yielded 72.22% positive for plasma or urine,and negative for all LCS samples.Conclusion: The rPCR has been optimized in this study with minimal DNA detectionat 50,000 copies/mL and was not cross-reacted with other microorganisms that arepotential to cause false positive results.;Background: Cytomegalovirus (CMV) is one of opportunistic infections in patientswith Aquired Immunodeficiency Syndrome (AIDS). Clinical manifestations are nottypical, and CT scans can not define encephalitis CMV specifically. Therefore, it isimportant to apply an alternative assay for sensitive and specific detection of CMVinfection in HIV patients with suspected central nervous system (CNS) infections.One of the assays is real time polymerase chain reaction (rPCR).Objective: To obtain a molecular assay for detection of CMV in HIV patients withsuspect CNS infections.Methods: This study was conducted in three phases. The first is optimization ofconcentrations of primers, probe, annealing temperature, final elution of DNAextraction, and volume of PCR template. The second is determinations of sensitivity(minimal detection of DNA) and specificity (cross-reaction) of the optimized rPCR,and the third is application of the rPCR for clinical samples of plasma, urine, andliquor cerebrospinal (LCS).Results: The rPCR reaction showed optimal concentrations of primers and probe at0.1 μM, with thermal cycler: 950C for 3 min (enzyme activation), followed by 45cycles of 950C for 15 sec (denaturation) and 560C for 1 min (annealing andextension). Final elution of DNA extraction was 40 μL and volume of PCR templatesfor urine, plasma, and LCS was 3, 4, and 5 μL, respectively. The rPCR had minimaldetection of DNA at 50,000 copies/mL and was not cross-reacted withStaphylococcus aureus, Staphylococcus epidermidis, Staphylococcus saprophyticus,Escherichia coli, Klebsiella pneumoniae, Pseudomonas aeruginosa, Mycobacteriumtuberculosis, Candida spp, Toxoplasma gondii, Epstein-Bar Virus (EBV), HerpesSimplex Virus (HSV) and Varicella Zoster Virus (VZV). Application of rPCR forclinical samples showed that the rPCR yielded 72.22% positive for plasma or urine,and negative for all LCS samples.Conclusion: The rPCR has been optimized in this study with minimal DNA detectionat 50,000 copies/mL and was not cross-reacted with other microorganisms that arepotential to cause false positive results.;Background: Cytomegalovirus (CMV) is one of opportunistic infections in patientswith Aquired Immunodeficiency Syndrome (AIDS). Clinical manifestations are nottypical, and CT scans can not define encephalitis CMV specifically. Therefore, it isimportant to apply an alternative assay for sensitive and specific detection of CMVinfection in HIV patients with suspected central nervous system (CNS) infections.One of the assays is real time polymerase chain reaction (rPCR).Objective: To obtain a molecular assay for detection of CMV in HIV patients withsuspect CNS infections.Methods: This study was conducted in three phases. The first is optimization ofconcentrations of primers, probe, annealing temperature, final elution of DNAextraction, and volume of PCR template. The second is determinations of sensitivity(minimal detection of DNA) and specificity (cross-reaction) of the optimized rPCR,and the third is application of the rPCR for clinical samples of plasma, urine, andliquor cerebrospinal (LCS).Results: The rPCR reaction showed optimal concentrations of primers and probe at0.1 μM, with thermal cycler: 950C for 3 min (enzyme activation), followed by 45cycles of 950C for 15 sec (denaturation) and 560C for 1 min (annealing andextension). Final elution of DNA extraction was 40 μL and volume of PCR templatesfor urine, plasma, and LCS was 3, 4, and 5 μL, respectively. The rPCR had minimaldetection of DNA at 50,000 copies/mL and was not cross-reacted withStaphylococcus aureus, Staphylococcus epidermidis, Staphylococcus saprophyticus,Escherichia coli, Klebsiella pneumoniae, Pseudomonas aeruginosa, Mycobacteriumtuberculosis, Candida spp, Toxoplasma gondii, Epstein-Bar Virus (EBV), HerpesSimplex Virus (HSV) and Varicella Zoster Virus (VZV). Application of rPCR forclinical samples showed that the rPCR yielded 72.22% positive for plasma or urine,and negative for all LCS samples.Conclusion: The rPCR has been optimized in this study with minimal DNA detectionat 50,000 copies/mL and was not cross-reacted with other microorganisms that arepotential to cause false positive results."

"Infeksi Hookworm (Necator americanus atau Ancylostoma duodenale) didunia mencapai sekitar 740 juta jiwa. Infeksi cacing tambang dapat menyebabkan malnutrisi, anemia dan defisiensi zat besi. Secara konvensional, diagnosis infeksi cacing tambang berdasarkan pada deteksi telur cacing tambang dalam sampel tinja manusia secara mikroskopik. Namun, metode tersebut memiliki beberapa keterbatasan. Terutama, seringnya kegagalan dalam membedakan sampai tingkat spesies. Dengan menggunakan Real Time PCR kita mengevaluasi infeksi submikroskopis hookwom (N. americanus dan A. duodenale) dari sampel feses anak (usia 5--18 tahun) pre dan post treatment Albendazole 400 mg di Nangapanda, Ende. Pemeriksaan dilakukan di Laboratorium Helmintologi, Departemen Parasitologi FKUI pada bulan November 2012 sampai dengan Mei 2013. Dua jenis probe spesifik yang digunakan dalam Real Time PCR: FAM dan Texas Red untuk mendeteksi N. americanus dan A. duodenale. Sebanyak 5 dari 90 sampel feses acak pre dan post treatment terinfeksi N. americanus dengan kandungan DNA rendah dan tidak ditemukan sampel yang terinfeksi A. duodenale. Penelitian menunjukkan bahwa Real Time PCR dapat mendeteksi infeksi submikroskopis spesies hookworm secara spesifik. Multiplex Real Time PCR sangat berguna untuk mendeteksi infeksi submikroskopis, terutama ketika intensitas infeksi rendah.

---

Hookworm infection (Necator americanus or Ancylostoma duodenale) in the world reachs about 740 million people. The infection of hookworm can lead to malnutrition, anemia and iron deficiency. Traditionally, diagnostic of hookworm infection is based on detection of hookworm eggs in human stool samples using microscopy. However, there are several limitations of this method. Importantly, species differentiation are often failed. Using Real Time PCR we evaluated submicroscopic infection of N. americanus and A. duodenale from human faecal samples (5-18years) in Nangapanda, Ende. The stool samples were collected in two times period, before and after treatment using 400mg of Albendazole. The examination was performed at the Laboratory of Parasitology,Faculty of Medicine Department Helmintologi during November 2012-May 2013. Two specific species probes were used in Real Time PCR: FAM and Texas Red to detect N.americanus and A.duodenale respectively. Five out of 90 random faecal samples were infected by N. americanus with low load DNA and none of A.duodenale infection was found. The present study shown that Real Time PCR could detect submicroscopic infection from specific species of hookworm. Multiplex Real Time PCR is very useful for detecting submicroscopic infections, especially when the intensity of hookworm infection is low."

"Nusa Tenggara Timur (NTT) merupakan salah satu provinsi dengan angka kekurangan nutrisi pada anak balita yang cukup tinggi. Kekurangan nutrisi merupakan penyebab mortalitas utama pada anak balita, yang dapat disebabkan oleh infeksi. Indonesia merupakan negara yang endemis terhadap soil transmitted helminth (STH) yang mencakup Ascaris lumbricoides, Trichuris trichiura, dan cacing tambang. Beberapa penelitian sebelumnya menunjukkan bahwa infeksi STH dapat menyebabkan kekurangan nutrisi pada anak. Oleh karena itu, penelitian ini bertujuan untuk mencari pengaruh infeksi STH terhadap kekurangan nutrisi pada anak balita di kecamatan Nangapanda, NTT yang diukur dengan weight-for-age z-score (WAZ), height-for-age z-score (HAZ), dan weight-for-height z-score (WHZ). Penelitian menggunakan desain cross-sectional dengan 98 subjek anak balita di Kecamatan Nangapanda yang berasal dari random sampling. Status WAZ, HAZ, dan WHZ diperoleh dari pengukuran antropometri, sementara status infeksi STH ditentukan melalui metode Kato-Katz untuk menemukan telur cacing di tinja. Hubungan antara infeksi STH dan kekurangan nutrisi pada anak balita dianalisis dengan chi-square, dan dilakukan analisis regresi logistik untuk mencari pengaruh faktor lain seperti usia anak balita, jenis kelamin, dan tingkat pendidikan ibu. Dari 98 anak balita, sebanyak 58 di antaranya terinfeksi STH. Sementara itu, ditemukan bahwa 27,6% anak balita memiliki WAZ <-2, 40,9% memiliki HAZ <-2, dan 10,2% memiliki WHZ <-2. Meskipun begitu, hasil analisis menunjukkan bahwa status infeksi STH tidak berhubungan secara bermakna dengan status gizi buruk pada anak balita, baik menurut WAZ (p = 0,997), HAZ (p = 0,244), maupun WHZ (p = 1,000). Analisis multivariat juga menunjukkan tidak terdapat hubungan yang signifikan dengan faktor lainnya. Oleh karena itu, dapat disimpulkan bahwa infeksi STH tidak mempengaruhi kekurangan nutrisi pada anak balita di NTT, sehingga diperlukan penelitian lebih lanjut.

---

East Nusa Tenggara Province had one of the highest rate of undernutrition in under-five children in Indonesia. Undernutrition contributes to a high proportion of mortality in under-five children, which can be caused by infection. Indonesia is endemic for soil-transmitted helminth (STH) infection, which can be caused by Ascaris lumbricoides, Trichuris trichiura¸ and hookworm. Several studies have shown that STH infections can cause malnutrition in under-five children. Therefore, this research aims to investigate the association between STH infection and undernutrition in under-five children measured by weight-for-age z-score (WAZ), height-for-age z-score (HAZ), and weight-for-height z-score (WHZ).

This is a cross-sectional study involving 98 under-five children which is recruited using random sampling from Nangapanda Sub-District, East Nusa Tenggara. WAZ, HAZ, and WHZ status is determined from anthropometry, while STH infections are determined by Kato-Katz method to find the helminth eggs. Chi-square analysis is performed to find the association between STH infection and nutritional status in under-five children, and logistic regression is also performed to find other potential factors such as age, gender, and mother?s education. Of the 98 children recruited, 58 had STH infections.

This study also found that 27,6% of the children had WAZ <-2, 40,9% had HAZ <-2, and 10,2% had WHZ <-2. However, chi-square analysis showed that there are no significant association between STH infection and undernutrition in under-five children of Nangapanda measured by WAZ (p = 0,997), HAZ (p = 0,244),and WHZ (p = 1,000). Multivariate analysis also showed that other factors in this study are not significant. Therefore, this research showed that STH infection are not the main cause of undernutrition in children of East Nusa Tenggara, and further research are warranted to determine other factors which may cause the problem."

"Ascaris lumbricoides termasuk kelompok nematoda usus yang dapat menimbulkan malnutrisi pada individu yang memiliki sistem imun lemah. Penelitian bertujuan untuk mendeteksi dan mengetahui persentase infeksi submikroskopis dari A. lumbricoides, dengan sampel feses anak usia 5-18 tahun di Nangapanda, menggunakan metode real-time PCR. Sampel feses dikoleksi selama dua kali, yaitu pre dan post treatment albendazole 400 mg. Total sampel yaitu 242, tetapi yang digunakan dengan uji real-time PCR hanya 45 sampel negatif secara mikroskopis. Sampel diisolasi kemudian dilakukan running realtime PCR. Primer yang digunakan berasal dari daerah target ITS-1. Daerah ITS-1 dipilih karena memiliki laju mutasi yang tinggi dan mampu menbedakan Ascaris dengan cacing lain. Real-time PCR mampu mendeteksi kuantitas DNA A. lumbricoides dalam jumlah yang sedikit. Deteksi sampel menggunakan realtime PCR menghasilkan kurva amplifikasi pada fluorophore VIC. Dua sampel (4,4%) pada pre treatment termasuk dalam low load of DNA (Ct > 35) dan lima sampel (11,4%) pada post treatment termasuk moderate load of DNA (30 < Ct < 35). Hasil penelitian menunjukkan bahwa real-time PCR dapat mendeteksi infeksi submikroskopis.

---

Ascaris lumbricoides is an intestinal nematode that can cause malnutrition, in the individual with weak immune system. The aim of this research is to detect and know the percentage of submicroscopic infection of A. lumbricoides, from human faecal samples (5-18 years) in Nangapanda by using real-time polymerase chain reaction (PCR) method. The faecal samples were collected in two times period, before and after treatment using 400 mg of Albendazole. Total samples were 242 but only 45 negative samples from microscopic detection were tested with realtime PCR. The samples were isolated and amplified with real-time PCR, by using primer from target area of internally transcribed spacer (ITS-1). ITS-1 region was chosen due to its high rate mutation and ability to differentiate Ascaris with the other helminth parasites. Real-time PCR can detect low load of A. lumbricoides DNA. Detection of samples with real-time PCR generated amplification curve in VIC fluorophore. Two samples (4.4%) in pre treatment were low load of DNA (Ct > 35) and five samples (11.4%) in post treatment were moderate load of DNA (30 < Ct < 35). The result showed that real-time PCR can detect submicroscopic infection of A. lumbricoides."

"Penelitian ini mengembangkan metode deteksi spesies babi (Sus scrofa) pada sampel daging campuran menggunakan automasi ekstraksi DNA magLEAD gC. DNA dianalisis menggunakan PCR dan TaqMan probe RT-PCR dengan primer spesifik untuk gen Cytochrome c oxidase I (COI), Cytochrome b (Cytb), dan NADH5 dehydrogenase 5 (ND5). Hasil menunjukkan bahwa ekstraksi DNA otomatis menghasilkan konsentrasi DNA 129,4–388,5 ng/μL pada daging mentah dan 66,4–89,5 ng/μL pada bakso dengan rasio kemurnian A260/A280 dan 260/A230 > 1,8. Primer COI, Cytb dan ND5 dapat mendeteksi DNA babi. PCR dan RT-PCR in vitro menunjukkan ketiga primer hanya mendeteksi DNA babi. Efisiensi amplifikasi RT-PCR primer COI, Cytb, dan ND5 adalah 144,14% (R2=0,982), 88,05% (R2=0,998), dan 81,25% (R2=0,997) dengan batas deteksi 0,0001 ng/μL, 0,001 ng/μL, dan 0,001 ng/μL. Primer/probe Cytb dan ND5 mendeteksi bakso dengan campuran daging babi hingga 0,1% (w/w).

---

This study developed a method to detect pig species (Sus scrofa) in mixed meat samples using automated DNA extraction with the magLEAD gC. DNA was analyzed using PCR and TaqMan probe RT-PCR with specific primers for the genes Cytochrome c oxidase I (COI), Cytochrome b (Cytb), and NADH5 dehydrogenase 5 (ND5). Results showed that automated DNA extraction produced DNA concentrations of 129.4–388.5 ng/μL in raw meat and 66.4–89.5 ng/μL in processed meatballs with purity ratios A260/A280 dan 260/A230 > 1.8. The COI, Cytb and ND5 primers could be used to detect pig DNA. In vitro PCR and RT-PCR showed that all three primers only detected pig DNA. The RT-PCR amplification efficiency for COI, Cytb, and ND5 primers were 144,14% (R2=0,982), 88,05% (R2=0,998), dan 81,25% (R2=0,997) with detection limits of 0.0001 ng/μL, 0.001 ng/μL, and 0.001 ng/μL. The Cytb and ND5 primers/probes detected meatballs with pig meat content as low as 0.1% (w/w)."

"Latar Belakang: Uveitis infeksi di Indonesia berkisar antara 30-60% dari total kasus uveitis. Identifikasi patogen etiologi infeksi sangat penting agar dapat diberikan terapi antimikroba yang sesuai dengan segera sehingga komplikasi kebutaan dapat diminimalisir. Dewasa ini, perkembangan teknologi biologi molekuler menggunakan metode Polymerase Chain Reaction (PCR) untuk deteksi uveitis infeksi sedang berkembang pesat.

Tujuan: Melakukan uji validasi diagnostik pada metode PCR Multiplex dibandingkan dengan metode PCR Tunggal.

Metodologi: Uji diagnostik untuk menentukan sensitivitas dan spesifisitas dari alat Real-Time PCR Multiplex terhadap PCR Tunggal dari spesimen cairan intraokular humor akuos yang diambil dari parasentesis bilik mata depan. Dilakukan pemeriksaan PCR terhadap patogen Mycobacterium tuberculosis (M.tuberculosis), Toxoplasma gondii (T.gondii), Herpes Simplex Virus (HSV), Varicella Zoster Virus (VZV), Cytomegalovirus, dan Treponema pallidum.

Hasil: Dilakukan analisis uji diagnostik pada 46 subjek penelitian. Didapatkan hasil sensitivitas sebesar 57.14% dan spesifisitas sebesar 100%. Positivity rate terbanyak didapatkan untuk patogen VZV (n=4), dan tidak didapatkan hasil positif terhadap deteksi patogen M.tuberculosis. Patogen T.pallidum berhasil dideteksi sebanyak 4.34% (n=2) oleh PCR Multiplex.

Kesimpulan: Metode PCR Multiplex pada penelitian ini memiliki sensitivitas yang rendah dengan spesifisitas yang tinggi. Hasil positif pada PCR Multiplex dapat bermanfaat untuk mendiagnosis pasien dengan uveitis infeksi.

---

Background: In Indonesia, infectious uveitis represents 30-60% of the country’s total uveitis cases. The identification of etiological pathogens is imperative to immediately select and administer the appropriate antimicrobial therapy in infectious uveitis, thereby complications of blindness can be minimized. Currently, the development of molecular biology technology using the Polymerase Chain Reaction (PCR) method for detection of infectious uveitis pathogens is growing rapidly.

Objective: To compare the diagnostic validation test results of the Multiplex PCR method and Single PCR method.

Method: Diagnostic test to determine the sensitivity and specificity of the Multiplex Real-Time PCR device against the Single PCR of aqueous humor intraocular fluid specimens taken from anterior chamber paracentesis. PCR examinations were carried out to identify the pathogens of Mycobacterium tuberculosis (M.tuberculosis), Toxoplasma gondii (T.gondii), Herpes Simplex Virus (HSV), Varicella Zoster Virus (VZV), Cytomegalovirus, dan Treponema pallidum.

Result: A diagnostic test analysis was performed on 46 study subjects. The results obtained 57.14% sensitivity and 100% specificity. Highest positivity rate was obtained for VZV pathogens, while positive results were not obtained for M.tuberculosis. There were 4.34% of subjects (n = 2) of T. pallidum were detected by PCR Multiplex. 

Conclusion: The PCR Multiplex method in this study has low sensitivity with high specificity. A positive result on Multiplex PCR can be useful for diagnosing patients with infectious uveitis."