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挪威云杉与毒蝇伞外生菌根中宿主上调和真菌磷酸果糖激酶活性下调的证据。

Evidence for an up-regulation of the host and a down-regulation of the fungal phosphofructokinase activity in ectomycorrhizas of Norway spruce and fly agaric.

作者信息

Schaeffer Christoph, Johann Patrik, Nehls Uwe, Hampp Rüdiger

机构信息

Physiological Ecology of Plants, Botanical Institute, University of Tübingen, Morgenstelle 1, D-72076 Tübingen, Germany.

出版信息

New Phytol. 1996 Dec;134(4):697-702. doi: 10.1111/j.1469-8137.1996.tb04935.x.

DOI:10.1111/j.1469-8137.1996.tb04935.x
PMID:33863202
Abstract

For an understanding of metabolic interactions in ectomycorrhizal associations it is essential to distinguish enzyme activities of the symbionts. For the ATP-dependent phosphofructokinase (PFK) from ectomycorrhizas of fly agaric (Amanita muscaria (L. ex Fr.) Hooker) on Norway spruce (Picea abies (L.) Karst.) we were able to achieve a symbiont-specific differentiation by special assay conditions. Substrate concentrations, Mg : ATP ratio and pH values which were optimum for the fly agaric PFK completely suppressed the PFK activity of spruce roots. On the other hand, under the optimum assay conditions for the spruce root PFK, the fungal PFK activity was reduced by more than 90%. The most pronounced difference between the enzymes of both organisms was the response towards fructose-2,6-bisphosphate (F26BP); whereas F26BP had no influence on the spruce PFK activity, the fly agaric PFK activity was strongly enhanced by very low levels of F26BP. The distinction of the partner-specific PFK activities illustrated that mycorrhiza formation exerted partner-specific effects. On the basis of host d. wt of the mycorrhizas, the host-specific PFK activity was more than doubled compared with that of the non-mycorrhizal short roots. By contrast, the fungal PFK activity, on a fungal d.wt basis, was reduced in the mycorrhizas to less than 1/4 of the activity of the free-living mycelium.

摘要

为了理解外生菌根共生体中的代谢相互作用,区分共生体的酶活性至关重要。对于来自挪威云杉(Picea abies (L.) Karst.)上的毒蝇伞(Amanita muscaria (L. ex Fr.) Hooker)外生菌根的ATP依赖性磷酸果糖激酶(PFK),我们能够通过特殊的测定条件实现共生体特异性分化。对毒蝇伞PFK而言最佳的底物浓度、Mg:ATP比值和pH值完全抑制了云杉根的PFK活性。另一方面,在云杉根PFK的最佳测定条件下,真菌PFK活性降低了90%以上。两种生物体的酶之间最显著的差异是对果糖-2,6-二磷酸(F26BP)的反应;F26BP对云杉PFK活性没有影响,而极低水平的F26BP会强烈增强毒蝇伞PFK的活性。伙伴特异性PFK活性的区分表明菌根形成产生了伙伴特异性效应。基于菌根宿主干重,宿主特异性PFK活性比非菌根短根增加了一倍多。相比之下,基于真菌干重,真菌PFK活性在菌根中降低到自由生活菌丝体活性的不到1/4。

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