Electrooptical properties of nucleic acids and nucleoproteins II. Study of the deoxyribonucleohistone-proflavine complexes

C. Houssier, E. Fredericq
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引用次数: 15

Abstract

The interaction between proflavine and the gel-forming deoxyribonucleohistone from calf thymus has been examined by means of the electrooptical method, in connexion with spectrophotometric, equilibrium dialysis and rigidity measurements, in media of very low ionic strenght.

  • 1.

    1. The changes in the visible and ultraviolet proflavine spectra were similar to those already mentioned by different authors for DNA and soluble deoxyribonucleohistone-proflavine complexes at higher ionic strenght. Only two important differences were observed: the isosbestic point was absent in the visible spectra and a slight shift (± 5 mμ) of the ultraviolet absorption band of the dye to shorter wavelengths was noticed.

  • 2.

    2. Binding curves showed an important interaction between proflavine and the gel-forming deoxyribonucleohistone in spite of the very low net electric charge of the macromolecule.

  • 3.

    3. The complexes displayed a negative dichroism in the visible range, due entirely to the dye. The dichroic ratio D increased with decreasing numbers of ligand molecules bound per atom of phosphorus (r) and reached a maximum value of about 1.85 (for r ⩽ 0.10), approximately constant in the whole visible absorption band (field strength: 13–13.5 kV/cm).

  • 4.

    4. At the same field strenght, the birefringence (B) at 550 mμ, per unit of gel-forming deoxyribonucleohistone concentration, increased towards a maximum value of about 1.45 dl/mg for r = 0.10.

  • 5.

    5. The birefringence relaxation times τ were not noticeably affected by the interaction except for r > 0.10 where a decrease of τ was observed.

The results are consistent with an intercalation of the proflavine cations between adjacent nucleotide pairs, for at most one proflavine molecule per five nucleotide pairs in the gel-forming deoxyribonucleohistone. For higher proflavine contents, the dye molecules “in excess” would be externally attached to the helix.

Some comparative measurements on a soluble-deoxyribonucleohistone fraction were in agreement with this scheme.

核酸和核蛋白的光电特性2。脱氧核糖核组蛋白-丙氨酸复合物的研究
用电光法,结合分光光度法、平衡透析法和刚性测量法,在极低离子强度的介质中研究了小牛胸腺中脯氨酸与凝胶形成的脱氧核糖核组蛋白之间的相互作用。1.1. 可见和紫外光谱的变化与不同作者已经提到的DNA和可溶性脱氧核糖核组蛋白-丙黄配合物在更高离子强度下的变化相似。只观察到两个重要的区别:在可见光谱中没有等吸点,并且注意到染料的紫外吸收带向较短波长轻微移位(±5 μ m)。结合曲线显示,尽管大分子的净电荷很低,但丙氨酸与成凝胶的脱氧核糖核组蛋白之间存在重要的相互作用。这些配合物在可见光范围内呈现负二色性,这完全是由于染料的作用。二向色比D随着每个磷原子结合的配体分子数(r)的减少而增加,达到最大值约为1.85 (r≥0.10),在整个可见吸收带(场强:13 ~ 13.5 kV/cm)内近似恒定。在相同的电场强度下,当r = 0.10.5.5时,每单位成胶脱氧核糖核组蛋白浓度为550 μ时的双折射(B)增加到1.45 dl/mg左右的最大值。除r >外,双折射弛豫时间τ不受相互作用的显著影响;0.10,观察到τ降低。在凝胶形成的脱氧核糖核组蛋白中,每五个核苷酸对中最多有一个丙氨酸分子,结果与相邻核苷酸对之间的丙氨酸阳离子插入一致。对于较高的脯氨酸含量,“过量”的染料分子会附着在螺旋的外部。对可溶性脱氧核糖核组蛋白组分的一些比较测量结果与该方案一致。
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