Jabben M, Shanklin J, Vierstra R D
Department of Horticulture, University of Wisconsin-Madison 53706.
J Biol Chem. 1989 Mar 25;264(9):4998-5005.
The plant photoreceptor chromoprotein, phytochrome, is rapidly degraded in vivo after photoconversion from a stable red light-absorbing form (Pr) to a far-red light-absorbing form (Pfr). Previously, we demonstrated that during Pfr degradation in etiolated oat seedlings, ubiquitin-phytochrome conjugates, (Ub-P), appear and disappear suggesting that phytochrome is degraded via a ubiquitin-dependent proteolytic pathway (Shanklin, J., Jabben, M., and Vierstra, R. D. (1987) Proc. Natl. Acad. Sci. U. S. A. 84, 359-363). Here, we provide additional kinetic and localization data consistent with this hypothesis by exploiting the unique ability to photoregulate phytochrome degradation in vivo. An assay for the quantitation of Ub-P was developed involving immunoprecipitation of total conjugates with anti-ubiquitin antibodies, followed by the detection of Ub-P with anti-phytochrome antibodies. Using this immunoassay, we found that Ub-P will accumulate to approximately 5% of initial phytochrome during Pfr degradation induced by a saturating red light pulse. Reducing the amount of Pfr produced initially by attenuating the red light pulse, lowered the amount of phytochrome degraded in the following dark period and concomitantly reduced the maximal accumulation of Ub-P. Continuous far-red irradiations that maintained only 4% of phytochrome as Pfr induced rapid phytochrome degradation similar to that induced by a red light pulse converting 86% of Pr to Pfr. The appearance and disappearance of Ub-P were similar for each irradiation indicating that Ub-P accumulation is independent of the level of Pfr provided rapid phytochrome degradation is maintained. Pulse-chase studies employing continuous far-red light followed by darkness showed that Ub-P are continuously synthesized during phytochrome degradation and rapidly disappear once degradation ceases. Ub-P also accumulated during "cycled Pr" degradation induced by the transformation of Pr to Pfr and back to Pr. The commitment to degrade cycled Pr and form Ub-P occurred within seconds after Pfr formation making the cause(s) underlying this phenomenon one of the fastest phytochrome reactions known. Within seconds after Pfr formation, a majority of phytochrome is also known to aggregate in vivo (previously defined as sequestered or pelletable), with aggregated phytochrome preferentially lost during phytochrome degradation. In vitro analysis of aggregated phytochrome indicated that they contain most of the Ub-P. Moreover, the appearance of Ub-P in the aggregated and soluble fractions correlated with the time that phytochrome disappeared from that fraction.(ABSTRACT TRUNCATED AT 400 WORDS)
植物光受体色素蛋白——光敏色素,在体内从稳定的吸收红光形式(Pr)光转换为吸收远红光形式(Pfr)后会迅速降解。此前,我们证明在黄化燕麦幼苗的Pfr降解过程中,泛素 - 光敏色素缀合物(Ub - P)出现又消失,这表明光敏色素是通过泛素依赖性蛋白水解途径降解的(尚克林,J.,贾本,M.,和维斯特拉,R. D.(1987年)美国国家科学院院刊84,359 - 363)。在此,我们通过利用体内光调节光敏色素降解的独特能力,提供了与该假设一致的更多动力学和定位数据。开发了一种定量Ub - P的测定方法,包括用抗泛素抗体免疫沉淀总缀合物,然后用抗光敏色素抗体检测Ub - P。使用这种免疫测定法,我们发现,在饱和红光脉冲诱导的Pfr降解过程中,Ub - P将积累至初始光敏色素的约5%。通过减弱红光脉冲来减少最初产生的Pfr量,降低了随后黑暗期降解的光敏色素量,并相应减少了Ub - P的最大积累量。仅将4%的光敏色素维持为Pfr的连续远红光照射诱导的光敏色素快速降解,类似于将86%的Pr转换为Pfr的红光脉冲诱导的降解。每次照射时Ub - P的出现和消失情况相似,表明只要维持快速的光敏色素降解,Ub - P的积累就与Pfr水平无关。采用连续远红光照射随后黑暗的脉冲追踪研究表明,在光敏色素降解过程中Ub - P持续合成,一旦降解停止就迅速消失。在由Pr转换为Pfr再转换回Pr诱导的“循环Pr”降解过程中,Ub - P也会积累。在Pfr形成后数秒内就会发生降解循环Pr并形成Ub - P,使得这一现象背后的原因成为已知最快的光敏色素反应之一。在Pfr形成后数秒内,还已知大多数光敏色素会在体内聚集(先前定义为隔离或可沉淀),聚集的光敏色素在光敏色素降解过程中优先丢失。对聚集的光敏色素的体外分析表明,它们含有大部分Ub - P。此外,聚集部分和可溶部分中Ub - P的出现与光敏色素从该部分消失的时间相关。(摘要截于400字)
