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mrna

Árabe

مرسال الحمض الريبي النووي

Última actualización: 2010-07-07
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Referencia: Wikipedia

Inglés

kits for purification of messenger ribonucleic acid mrna

Árabe

مجموعات لتنقية الحمض النووي الريبي الرسول

Última actualización: 2018-07-23
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Inglés

52. mrna therapeutics has seen continued commercialization.

Árabe

52- ويتواصل إضفاء الطابع التجاري على المداواة المرتبطة بالحمض النووي الريبي المرسال().

Última actualización: 2016-12-01
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Referencia: Drkhateeb

Inglés

*transcription and mrna splicing - gene expression.

Árabe

* نسخ وراثي وmrna splicing - التعبير الجيني.

Última actualización: 2016-03-03
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Referencia: Drkhateeb

Inglés

we received the results from the mrna sequences this morning.

Árabe

لقد تلقينا نتائج من جهازالتتبعالنوويفيصباح اليوم...

Última actualización: 2016-10-27
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Referencia: Drkhateeb

Inglés

kits for messenger ribonucleic acid mrna quantitation by polymerase chain reaction pcr

Árabe

أنظمة تحديد وسيط الكميات للحمض نووي ريبي عن طريق سلسلة التفاعل البلمرة بي سي ار

Última actualización: 2018-07-23
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Referencia: Drkhateeb

Inglés

production of mrna is initiated by proteins known as transcription factors.

Árabe

ويبدأ إنتاج الـ mrna بواسطة بروتينات تعرف باسم عوامل النسخ.

Última actualización: 2016-03-03
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Referencia: Drkhateeb

Inglés

the test result is currently reported as a specimen ratio of pca3 mrna to psa mrna.

Árabe

نتيجة الاختبار معروفة في الوقت الحالي كنتيجة اختبارية بين pca3 mrna و psa mrna .

Última actualización: 2016-03-03
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Inglés

ace2 mrna expression is also found in the cerebral cortex, striatum, hypothalamus, and brainstem.

Árabe

الحمض النووي الريبوزي المرسال الخاص بالإنزيم المحول للأنجيوتنسين 2 موجود في القشرة الدماغية، والمخطط، ومنطقة تحت المهاد، وجذع الدماغ.

Última actualización: 2020-08-25
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Referencia: Drkhateeb

Inglés

pfizer has received your order for comirnaty (covid-19 mrna vaccine).

Árabe

تلقت شركة pfizer طلبكم للحصول على كوميرناتي (لقاح مصنّع من مرسال الحمض الريبي النووي لفيروس كورونا).

Última actualización: 2021-01-30
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Referencia: Drkhateeb
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Inglés

" demonstrated that the extra sequence in the yeast gene was transcribed into mrna and removed itself from the host protein only after translation.

Árabe

وفي 1990 برهن هيراتا وغيره بأن التسلسل الزائد في جين الخميرة استحال إلى رنا مرسال وأزال نفسه من البروتين المضيف بعدما تمت عملية الترجمة فقط.

Última actualización: 2016-03-03
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Referencia: Drkhateeb
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Inglés

positive-sense viral rna is in the same sense as viral mrna and thus at least a part of it can be immediately translated by the host cell.

Árabe

الرنا الفيروسي موجب الاتجاه يكون في نفس اتجاه مرسال الحمض الريبي النووي الفيروسي وبالتالي يمكن فوراً ترجمت جزء منه على الأقل من قبل الخلية المضيفة.

Última actualización: 2016-03-03
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Referencia: Drkhateeb

Inglés

on 17 march 2020, american pharmaceutical company pfizer announced a partnership with german company biontech to jointly develop a mrna-based vaccine.

Árabe

في 17 مارس 2020، أعلنت شركة الأدوية الأمريكية pfizer عن شراكة مع شركة biontech الألمانية للاشتراك في تطوير لقاح قائم على الحمض النووي الريبوزي المرسال.

Última actualización: 2020-08-25
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Referencia: Drkhateeb

Inglés

metabolic variables and basal substrate kinetics basal glucose and fatty acid kinetics. basal glucose and palmitate kinetics were not different between matched subjects within any of the 2 groups (table 2). insulin sensitivity. hepatic (fig. 1a), skeletal muscle (fig. 1b), and adipose tissue (fig. 1c) insulin sensitivity was lower in subjects with high than in those with normal ihtg content. however, no differences in insulin sensitivity measures were observed between subjects with low or high vat volume, when matched on ihtg content (fig. 1). fig. 1. fig. 1. hepatic (a), skeletal muscle (b), and adipose tissue (c) insulin sensitivity in subjects matched on visceral adipose tissue (vat) volume with either normal or high intrahepatic triglyceride (ihtg) content and subjects matched on ihtg content who had either ... vldl-tg kinetics. hepatic vldl-tg secretion rate was almost double in subjects with high than in those with normal ihtg content (23 ± 2 and 12 ± 1 μmol/min, respectively; p 10% of liver volume) (n = 10) or normal (≤5.5% of liver volume) (n = 10) ihtg content (table 1) (41). the range in vat volume was similar in both the normal (vat volume: 689–3,088 cm3) and the high (vat volume: 638–2,702 cm3) ihtg groups. each subject with normal ihtg and a given vat volume was matched with a subject from the high ihtg group on vat (within ≈20% of vat volume of the normal ihtg group). group 2 subjects (n = 20) were matched on ihtg content and had either low (n = 10) or high (n = 10) vat volume (table 1). subjects were separated into low and high vat volume groups by using the median value of all subjects (1,100 cm3) as the cut point for low and high vat volumes. subjects within groups were matched on age, sex, bmi, and percentage of body fat. we did not have knowledge of any outcome measures when the matches were performed. all subjects completed a comprehensive medical evaluation, which included a 2-h oral glucose tolerance test. no subject had any history or evidence of liver disease other than nafld, took medications that can affect metabolism or cause hepatic abnormalities, consumed >20 g/day of alcohol, or had diabetes. subjects gave their written informed consent before participating in this study, which was approved by the human research protection office of washington university school of medicine, st. louis, mo. body composition analyses. body fat mass (fm) and fat-free mass (ffm) were determined by using dual-energy x-ray absorptiometry (delphi-w densitometer, hologic). intraabdominal and abdominal s.c. adipose tissue volumes were quantified by magnetic resonance imaging (siemens; analyze 7.0 software, mayo foundation) (9) and ihtg content was measured by using proton magnetic resonance spectroscopy (siemens) as we have previously described (42). hyperinsulinemic–euglycemic clamp procedure. subjects were admitted to the intensive research unit at washington university school of medicine on the evening before the clamp procedure. at 0500 hours the following morning, after subjects fasted for 12 h overnight, a 2-stage hyperinsulinemic–euglycemic clamp procedure was started and continued for 9 h. insulin was infused at a rate of 20 mu·m−2 body-surface area (bsa)·min−1 during stage 1 (3–6 h) and at a rate of 50 mu·m−2 bsa·min−1 during stage 2 (6–9 h) of the clamp procedure (9, 43). [6,6-2h2]glucose, [2,2-2h2]palmitate, and 20% dextrose enriched to 2.5% with [6,6-2h2]glucose were infused to determine hepatic, skeletal muscle, and adipose tissue insulin sensitivity. tissue samples were obtained from s.c. abdominal adipose tissue and from the quadriceps femoris muscle 60 min after starting the glucose tracer infusion during the basal stage. a detailed description of the infusion protocol and of collection of tissues and blood samples is available in supporting information (si) materials and methods. vldl-tg kinetics study. one week after the hyperinsulinemic–euglycemic clamp procedure, subjects were readmitted to the intensive research unit on the evening before the vldl kinetics study. at 0600 hours the following morning, after subjects fasted for 12 h overnight, a bolus of [1,1,2,3,3-2h5]glycerol was injected, and a constant infusion of 2,2-2h2]palmitate was started and main

Árabe

metabolic variables and basal substrate kinetics basal glucose and fatty acid kinetics. basal glucose and palmitate kinetics were not different between matched subjects within any of the 2 groups (table 2). insulin sensitivity. hepatic (fig. 1a), skeletal muscle (fig. 1b), and adipose tissue (fig. 1c) insulin sensitivity was lower in subjects with high than in those with normal ihtg content. however, no differences in insulin sensitivity measures were observed between subjects with low or high vat volume, when matched on ihtg content (fig. 1). fig. 1. fig. 1. hepatic (a), skeletal muscle (b), and adipose tissue (c) insulin sensitivity in subjects matched on visceral adipose tissue (vat) volume with either normal or high intrahepatic triglyceride (ihtg) content and subjects matched on ihtg content who had either ... vldl-tg kinetics. hepatic vldl-tg secretion rate was almost double in subjects with high than in those with normal ihtg content (23 ± 2 and 12 ± 1 μmol/min, respectively; p 10% of liver volume) (n = 10) or normal (≤5.5% of liver volume) (n = 10) ihtg content (table 1) (41). the range in vat volume was similar in both the normal (vat volume: 689–3,088 cm3) and the high (vat volume: 638–2,702 cm3) ihtg groups. each subject with normal ihtg and a given vat volume was matched with a subject from the high ihtg group on vat (within ≈20% of vat volume of the normal ihtg group). group 2 subjects (n = 20) were matched on ihtg content and had either low (n = 10) or high (n = 10) vat volume (table 1). subjects were separated into low and high vat volume groups by using the median value of all subjects (1,100 cm3) as the cut point for low and high vat volumes. subjects within groups were matched on age, sex, bmi, and percentage of body fat. we did not have knowledge of any outcome measures when the matches were performed. all subjects completed a comprehensive medical evaluation, which included a 2-h oral glucose tolerance test. no subject had any history or evidence of liver disease other than nafld, took medications that can affect metabolism or cause hepatic abnormalities, consumed >20 g/day of alcohol, or had diabetes. subjects gave their written informed consent before participating in this study, which was approved by the human research protection office of washington university school of medicine, st. louis, mo. body composition analyses. body fat mass (fm) and fat-free mass (ffm) were determined by using dual-energy x-ray absorptiometry (delphi-w densitometer, hologic). intraabdominal and abdominal s.c. adipose tissue volumes were quantified by magnetic resonance imaging (siemens; analyze 7.0 software, mayo foundation) (9) and ihtg content was measured by using proton magnetic resonance spectroscopy (siemens) as we have previously described (42). hyperinsulinemic–euglycemic clamp procedure. subjects were admitted to the intensive research unit at washington university school of medicine on the evening before the clamp procedure. at 0500 hours the following morning, after subjects fasted for 12 h overnight, a 2-stage hyperinsulinemic–euglycemic clamp procedure was started and continued for 9 h. insulin was infused at a rate of 20 mu·m−2 body-surface area (bsa)·min−1 during stage 1 (3–6 h) and at a rate of 50 mu·m−2 bsa·min−1 during stage 2 (6–9 h) of the clamp procedure (9, 43). [6,6-2h2]glucose, [2,2-2h2]palmitate, and 20% dextrose enriched to 2.5% with [6,6-2h2]glucose were infused to determine hepatic, skeletal muscle, and adipose tissue insulin sensitivity. tissue samples were obtained from s.c. abdominal adipose tissue and from the quadriceps femoris muscle 60 min after starting the glucose tracer infusion during the basal stage. a detailed description of the infusion protocol and of collection of tissues and blood samples is available in supporting information (si) materials and methods. vldl-tg kinetics study. one week after the hyperinsulinemic–euglycemic clamp procedure, subjects were readmitted to the intensive research unit on the evening before the vldl kinetics study. at 0600 hours the following morning, after subjects fasted for 12 h overnight, a bolus of [1,1,2,3,3-2h5]glycerol was injected, and a constant infusion of 2,2-2h2]palmitate was started and main

Última actualización: 2021-04-15
Frecuencia de uso: 3
Calidad:

Referencia: Drkhateeb
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