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天然丰度碳-13傅里叶变换核磁共振谱及未分级酵母转移核糖核酸的自旋晶格弛豫时间

Natural-abundance carbon-13 Fourier-transform nuclear magnetic resonance spectra and spin lattice relaxation times of unfractionated yeast transfer-FNA.

作者信息

Komoroski R A, Allerhand A

出版信息

Proc Natl Acad Sci U S A. 1972 Jul;69(7):1804-8. doi: 10.1073/pnas.69.7.1804.

Abstract

High-resolution Fourier-transform nuclear magnetic resonance at 15.18 MHz was used to observe the proton-decoupled natural-abundance (13)C spectra of aqueous unfractionated tRNA from baker's yeast in the presence of Mg(+2) (8 ions per tRNA molecule), as a function of temperature in the range of 27-82 degrees C. The spectrum of thermally denatured tRNA at 82 degrees C showed numerous sharp resonances, which were assigned to specific types of carbon atoms by comparison with the (13)C spectra of mononucleotides. Only the resonance of carbon 4' of the ribose rings was appreciably shifted (by about 1.5 ppm upfield) with its average position in the mononucleotides. This effect was also seen in the spectrum of poly(A). In the spectrum of folded tRNA (52 degrees C), carbon 4' was further shifted upfield by about 1.5 ppm, and carbons 2' and 3', which yielded a single resonance at 82 degrees C, now showed two partly resolved peaks. The variation of linewidths with temperature (200 mg/ml of tRNA) was gradual in the range 27-82 degrees C, and did not reflect the expected unfolding behavior of tRNA. Moreover, dilution to 80 mg/ml at 27 degrees C had the same effect as an increase in temperature to about 45 degrees C. The line-width changes below 60 degrees were ascribed to tRNA aggregation. In contrast to the behavior of the linewidths, the (13)C spin-lattice relaxation times (T(1)) of individual ribose carbon atoms, measured by means of partially relaxed Fourier-transform spectra were practically independent of temperature up to about 60 degrees C, and increased rapidly at higher temperatures. The T(1) values indicated that the backbone of thermally denatured tRNA is undergoing rapid segmental motion, with an effective correlation time of (2.6 +/- 0.5) x 10(-10) sec. The T(1) values of folded tRNA yielded no evidence of segmental motion. The correlation time for overall rotational reorientation is about (3 +/- 1) x 10(-8) sec in the range 35-54 degrees C. Within experimental error, the T(1) values of methine carbons of the bases were equal to those of the methine carbons on the backbone at all temperatures. Only an upper limit to the rate of internal rotation of the bases could be established.

摘要

在镁离子(每个tRNA分子8个离子)存在的情况下,使用15.18兆赫兹的高分辨率傅里叶变换核磁共振来观察来自面包酵母的未分级水性tRNA的质子去耦自然丰度(13)C谱,作为27至82摄氏度范围内温度的函数。82摄氏度下热变性tRNA的谱显示出许多尖锐的共振峰,通过与单核苷酸的(13)C谱比较,这些共振峰被归属于特定类型的碳原子。只有核糖环的4'碳的共振峰有明显位移(向上场约1.5 ppm),其在单核苷酸中的平均位置也如此。这种效应在聚(A)的谱中也可见。在折叠tRNA(52摄氏度)的谱中,4'碳进一步向上场位移约1.5 ppm,并且在82摄氏度时产生单一共振峰的2'和3'碳,现在显示出两个部分分辨的峰。在27至82摄氏度范围内,线宽随温度(200毫克/毫升tRNA)的变化是逐渐的,并且没有反映出tRNA预期的解折叠行为。此外,在27摄氏度下稀释至80毫克/毫升与温度升高至约45摄氏度具有相同的效果。60摄氏度以下的线宽变化归因于tRNA聚集。与线宽的行为相反,通过部分弛豫傅里叶变换谱测量的各个核糖碳原子的(13)C自旋晶格弛豫时间(T(1))在高达约60摄氏度时实际上与温度无关,并且在较高温度下迅速增加。T(1)值表明热变性tRNA的主链正在经历快速的片段运动,有效相关时间为(2.6±0.5)×10(-10)秒。折叠tRNA的T(1)值没有显示出片段运动的证据。在35至54摄氏度范围内,整体旋转重取向的相关时间约为(3±1)×10(-8)秒。在实验误差范围内,所有温度下碱基次甲基碳的T(1)值与主链上次甲基碳的T(1)值相等。只能确定碱基内旋转速率的上限。

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