6 research outputs found

    A 22 q11.2 deletion case with multiorgan failure

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    The 22q11.2 deletion syndrome is a genetic disorder seen inone out of every 4,000-6000 live births. The effects of the deletion can include a variety of physical findings, such as heart problems, cleft palate, facial dysmorphism, tymic hypoplasia, hypocalcemia, immune deficiency, developmental issues, including learning difficulties. The case was the second born child of 33 year old healthy mother by Caesarian section at 37 weeks of gestation. Birth weight of the baby girlwas 3400 g. She was referred to our unit on her first day due to respiratory distress. She had diffuse edema, cutis marmoratus and low set ears. Her oral orifice was small and the mouth was pulled downward on one side while crying. She was tachypneic, grunting. She had cyanosis, retractions, nasal flaring and hepatomegaly. Femoral pulses were weak. She had hypocalcemia, metabolic acidosis, hyperuricemia, hyperkalemia, abnormal renal function tests. Thymic shadow was absent on chest x-ray. Thrombocytopenia and giant thrombocytes were seen on peripheral blood smear. PTH level was normal. Interrupted aortic arch type-B was detected by echocardiographic examination and prostoglandin infusion was started. 22q11.2 deletion was detected by FISH examination. Interrupted aortic arch cases may be present with metabolic acidosis, edema, hepatomegaly and multiorgan failure during newborn period. 22q11 deletion should be considered in interrupted aortic arch cases with accompanying features such as characteristic facial appearance, thymic aplasia, hypocalcemia, giant thrombocytes and surgical team should be informed

    Akut lenfoblastik lösemi hastalarında t(4;11) MLL/AF4 translokasyonunun real time RT-PCR ile 5 yıllık sonuçlarının retrospektif değerlendirilmes

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    Aim: t(4,11) is a chromosomal abnormality formed by the translocation MLL-AF4, which is the result of the fusion of the AF4 gene, localized on 4q21 chromosomal band, to the MLL gene, localized on 11q23 chromosomal band. The aim of this study is to examine the results of the analysis of t (4;11) MLL-AF4 translocation in acute lymphoblastic leukemia (ALL) patients retrospectively. Materials and Methods: Peripheral blood or bone marrow samples of 176 children (70 girls, 106 boys) and 144 adults (60 women, 84 men) with a preliminary diagnosis of acute leukemia between 2009-2013 were analyzed in the Medical Biology Department of Ege University Faculty of Medicine. The translocation RNA results of 71 peripheral blood and 473 bone marrow samples of these patients were evaluated quantitatively for t(4;11) with real-time RT- PCR. t(4;11) quantitation was performed by real-time qRT-PCR instrument after the synthesis of complementary DNA with conventional PCR from total RNA or mRNA isolated from blood and bone marrow. Quantitative analysis of the patients was performed by comparing positive and negative controls and samples classified as positive or negative (the ratio of the number of positive copies to the number of reference copies). Results: A total of 320 patients, with 98 having also follow-ups, were evaluated for t(4;11) translocation. Totally 34 patients (24 children and 10 adults) were found positive and the other samples were negative. Conclusion: The assessment of these results supports that, quantitative determination of t(4;11) with RT-PCR method among newly diagnosed ALL patients and ALL patients undergoing treatment, is a valuable method for both confirming the diagnosis and guiding the treatment intended to achieve molecular remission.Amaç: t(4;11), MLL-AF4 translokasyonu sonucu oluşan, 4q21 kromozomal bandına yerleşim gösteren AF4 geninin 11q23 kromozomal bandına yerleşim gösteren MLL genine füzyonu sonucu gelişen kromozomal bir anomalidir. Bu çalışmada, retrospektif olarak 2009-2013 yılları arasındaki akut lenfoblastik lösemi (ALL) hastalarındaki t(4;11) MLL- AF4 translokasyonunun analiz sonuçlarının incelenmesi amaçlandı. Gereç ve Yöntem: Ege Üniversitesi Tıp Fakültesi Tıbbi Biyoloji Anabilim Dalı’na 2009-2013 yılları arasında akut lösemi ön tanısıyla 176 çocuk (70 kız, 106 erkek) ve 144 yetişkin (60 kadın, 84 erkek) olgunun kan veya kemik iliği örnekleri incelendi. Bu olgulara ait 71 kan ve 473 kemik iliği örneğinin t(4;11) translokasyon RNA sonuçları, gerçek zamanlı RT-PCR yöntemi ile kantitatif olarak değerlendirildi. İlk aşamada, kan ve kemik iliği örneklerinden izole edilen total RNA veya mRNA’dan konvansiyonel bir PCR cihazı ile komplementer DNA sentezlendi. İkinci aşamada, gerçek zamanlı PCR cihazı ile t(4;11) kantitasyonu gerçekleştirildi. Olguların kantitatif olarak değerlendirilmesi, pozitif kontrol ve negatif kontrolün karşılaştırılması ile örneklerin negatif yada pozitif (pozitif olgu kopya sayısının referans kopya sayısına oranı) olması şeklinde yapıldı. Bulgular: Çalışmamızda 98’i takip hastası olmak üzere toplam 320 hasta t(4;11) MLL-AF4 translokasyonu için değerlendirildi. Çalışmaların sonucunda toplam 34 olgu (24 çocuk, 10 yetişkin) pozitif ve diğer örnekler negatif olarak bulundu. Sonuç: Bu değerlendirmenin sonuçları, RT-PCR yöntemi ile ALL hastalarında yeni tanı döneminde ve tedavi sürecinde t(4;11) MLL-AF4 translokasyonunun kantitatif tayini, hem tanının kesinleştirilmesinde hem de moleküler remisyon sağlanmasına yönelik tedaviyi yönlendirmesinde değerli bir yöntem olduğunu desteklemektedir
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