Effects of Temperature on the Circadian Conidiation Rhythm of Temperature-Sensitive Mutants of Neurospora crassa

Period lengths at different temperatures and phase responsecurves at a high temperature (35°C) of circadian conidiationrhythms were examined in 13 temperature-sensitive (un) strainsof Neurospora crassa. Two strains, un-16 and un-18, had longerperiod lengths than the wild-type strain even at permissivetemperatures. Period lengths of six strains, un-4, un-11, un-16,un-18, un-19 and un-22, changed differently from that of thewild-type strain at restrictive temperatures. However, the shapeof phase response curves for high temperature (35°C) for3 h was almost the same for all un strains and the wild-typestrain. We isolated 97 temperature-sensitive mutants with periodlengths from 19.2 to 24.8 h and determined the dependence ontemperature of the period length of the conidiation rhythm foreach mutant. The mutants could be divided into four differentgroups in terms of their responses to changes in temperature. (Received September 8, 1993; Accepted March 10, 1994)     

Spatial Distribution of Circadian Clock Phase in Aging Cultures of Neurospora crassa

Neurospora crassa has been utilized extensively in the study of circadian clocks. Previously, the clock in this organism has been monitored by observing the morphological and biochemical changes occurring at the growing front of cultures grown on solid medium. A method has been developed for assaying the clock in regions of the culture behind the growing front, where no apparent morphological changes occur during the circadian cycle. Using this assay with Petri dish cultures that were 2 to 7 days old, the presence of a functional circadian clock not only at the growing front but in all other regions of the culture as well was demonstrated. Furthermore, the entire culture is not in the same phase, but shows a gradient of phases which is a function of the length of time the clock in a given part of the culture has been free-running. This gradient may be the result of a somewhat longer period of the oscillator behind the growing front compared to that at the growing front. The phase differences within a single culture of interconnected mycelium demonstrate the absence of total internal synchronization between adjacent regions of the hyphae under these conditions.     

Cold-sensitive Mutants of Neurospora crassa

Cold-sensitive mutants of the eucaryote Neurospora crassa have been isolated by a modification of the filtration-enrichment technique of Catcheside. The mutants include osmotic remedial, auxotrophic, transport, and incorporation deficient isolates.     

粗糙脉孢菌及其他真菌中生物钟系统研究进展

地球自转形成的昼夜交替促使地球上的生物在体内进化出了能够测量时间的"生物钟"系统,此系统由输入途径、核心振荡器和输出途径3部分组成。"光逃避"假说为生物钟的进化提供了一种合理的解释。作为研究生物钟的理想模式生物之一,粗糙脉孢菌生物钟的核心振荡器是由正调控因子WC-1、WC-2和负调控因子FRQ、FRH组成的一个基于转录/翻译的负反馈调控环路。输入途径感知光照、温度等环境信号并将其传递到核心振荡器,进而调控下游一系列钟控基因表达,输出昼夜节律。此外,粗糙脉孢菌中还存在不依赖于WC复合体的frq基因的转录,其调控方式的解析进一步丰富了生物钟的调控网络。最后,通过比较并探索其他真菌中生物钟系统组成及运行机制,使我们对真菌生物钟的进化历程及生物体对环境的整体适应性有了更加全面而深刻的认识。     

Phase Shifting of the Circadian Clock by Diethylstilbestrol and Related Compounds in Neurospora crassa

Phase shifts of the circadian conidiation rhythm in Neurospora crassa were induced by 3-hour treatments of mycelia in liquid medium with diethylstilbestrol (DES), dienestrol (DIE), hexestrol (HEX), diethylstilbestroldipropionate (DESP), and dienestroldiacetate (DIEA). Over a 24-hour period beginning 24 hours after the transition from light to constant dark, maximum phase shifts occurred about 36 hours. DES was the most effective of the drugs tested, giving 10-hour phase advances at 20 micromolar. DIE and HEX caused similar phase shifts as DES at 40 micromolar. The two derivatives of the last, DESP and DIEA, were much less effective in shifting phase; only a few hours of phase advance result from treatments at 80 micromolar concentrations.

The activity of isolated plasma membrane ATPase was inhibited by DES and partially by HEX, but not by DIE, DESP, or DIEA. O₂ consumption of the mycelia was inhibited equally by DES, DIE, and HEX, while DIEA and DESP had little effect. Phase-shifts by DES cannot be interpreted as evidence that plasma membrane ATPase is a component of the circadian clock.

     

Mutants affecting thymidine metabolism in Neurospora crassa

When (14)C-thymidine labeled only in the ring is administered to Neurospora crassa, the majority of the recovered label is found in the ribonucleic acid (RNA). Three mutants were isolated in which different steps are blocked in the pathway that converts the pyrimidine ring of thymidine to an RNA precursor. Evidence from genetic, nutritional, and accumulation studies with the three mutants shows the pathway to proceed as follows: thymidine --> thymine --> 5-hydroxymethyluracil --> 5-formyluracil --> uracil --> uridylic acid. A mutant strain in which the thymidine to thymine conversion is blocked is unable to metabolize thymidine appreciably by any route, including entry into nucleic acids. This suggests that Neurospora lacks a thymidine phosphorylating enzyme. A second mutation blocks the pathway at the 5-hydroxymethyluracil to 5-formyluracil step, whereas a third prevents utilization of uracil and all compounds preceding it in the pathway. The mutant isolation procedures yielded three other classes of mutations which are proposed to be affecting, respectively, regulation of the thymidine degradative pathway, transport of pyrimidine free bases, and transport of pyrimidine nucleosides.     

Selection of Respiratory Mutants of Neurospora crassa

A method is described that permits the isolation of mutants that are defective in mitochondrial respiration. The techniques of inositol-less death and overlay with 2,3,5-triphenyl-2H-tetrazolium chloride are utilized to select for mutant colonies. Colonies that survive inositol-less death and fail to reduce the tetrazolium dye are then tested polarographically for cyanide-sensitive respiration. A preliminary characterization of three mutants obtained by this method is presented. The mutants have been characterized by their cyanide-sensitive respiration rate, growth rate, the state III respiration rate of isolated mitochondria, inhibition of the respiration of isolated mitochondria by cyanide and antimycin A, and cytochrome spectra. All of the mutants described differ from the parent strain in some of these aspects.     

Effects of Membrane ATPase Inhibitors on Light-Induced Phase Shifting of the Circadian Clock in Neurospora crassa

Effects of several membrane ATPase inhibitors on light-induced phase shifting of the circadian conidiation rhythm in Neurospora crassa were examined using mycelial discs in liquid culture. Suppression of phase shifting by the inhibitors was strongly dependent on the pH of the liquid medium in which the discs were cultured during the time from light-dark transition (beginning of free-run) to light irradiation. When discs were cultured in pH 6.7 medium, azide, the inhibitors of plasma membrane ATPase (diethylstilbestrol and N, N′-dicyclohexylcarbodiimide), and ethanol completely suppressed the effect of light on the clock. In contrast, mycelial discs cultured in pH 5.7 medium were fully phase-shifted by light in the presence of the same and even higher concentrations of the chemicals. However, sensitivity to light of the discs cultured in relatively acidic medium was eight times higher than that of the discs cultured at neutral pH. Oligomycin and venturicidin, inhibitors of mitochondrial ATPase, did not suppress phase shifting by light at either pH.     

A Liquid Culture Method for the Biochemical Analysis of the Circadian Clock of Neurospora crassa

The circadian clock that regulates the conidiation rhythm ofNeurospora crassa has been reported to function normally inliquid cultures, even if they make almost no conidia and growpoorly. The phase of the rhythm was not affected by a transferfrom liquid to solid medium [Perlman et al. (1981) Plant Physiol.in press]. These studies used a pantothenate-requiring auxotroph.This report describes a similar liquid culture method, in whichthere is no growth or conidiation and no phase shift causedby the transfer from a liquid to solid medium, and in whichthe wild type (bd) strain is used. Conidia were germinated inliquid medium containing glucose and arginine at the usual concentrationsin continuous light. After 33 hr, discs were cut from the hyphalmats with a cork borer and transferred to liquid medium containingglucose and arginine at concentrations ten times lower thanusual, then the discs were immediately placed in continuousdarkness with shaking. About 18 hr after the light-dark transition,growth stopped completely and respiratory activity was suppresseddue to the depletion of exogenous carbon source. No conidiawere visible. But, the clock functioned normally for at least60 hr because the phase of the rhythm of the race tubes inoculatedwith experimental discs was very similar to the phase of thediscs which had been transferred to solid medium without culturein the low-carbon-source liquid medium. Sensitivity to perturbationby light and to cycloheximide pulse treatments also changedrhythmically. Both are evidence of normal functioning of theclock in the liquid medium. This liquid culture method willbe useful for studying the biochemical mechanism of the circadianclock. (Received October 30, 1980; Accepted December 18, 1980)     

Mutants with Altered Sensitivity to a Calmodulin Antagonist Affect the Circadian Clock in Neurospora Crassa

Two newly isolated mutant strains of Neurospora crassa, cpz-1 and cpz-2, were hypersensitive to chlorpromazine with respect to mycelial growth but responded differently to the drug with respect to the circadian conidiation rhythm. In the wild type, chlorpromazine caused shortening of the period length of the conidiation rhythm. Pulse treatment with the drug shifted the phase and inhibited light-induced phase shifting in Neurospora. By contrast to the wild type, the cpz-2 strain was resistant to these inhibitory effects of chlorpromazine. Inhibition of cpz-2 function by chlorpromazine affected three different parameters of circadian conidiation rhythm, namely, period length, phase and light-induced phase shifting. These results indicate that the cpz-2 gene must be involved in or related closely to the clock mechanism of Neurospora. By contrast, the cpz-1 strain was hypersensitive to chlorpromazine with respect to the circadian conidiation rhythm.     

Free Cellular Riboflavin is Involved in Phase Shifting by Light of the Circadian Clock in Neurospora crassa

Phase shifting by light of the circadian conidiation rhythmof the Neurospora crassa strain band, of the riboflavin-deficientdouble mutant band rib2 and of the temperature-sensitive doublemutant band ribl was measured. Fluence response curves of theband strain exhibited two distinct steps, whereas those of bandribl and band rib2 revealed only one step. Maximum phase advancesobserved were 5.5 h in band and 10.4 h in the band rib strains.Sensitivity of band rib2 to light was proportional to the riboflavinconcentration in the growth medium over a 100 fold range. Extracellularflavin in the medium did not sensitize the strains. Riboflavinapplied after exposure to light showed no effect. Light sensitivitycorrelated with the level of cellular riboflavin. Four analogsof riboflavin, none of which can be phosphorylated, increasedthe sensitivity of Neurospora to light. Even at high riboflavinconcentrations in the medium, the sensitivity of the band rib2strain to light was not saturated. In addition, four riboflavinderivatives with bulky substituents at positions 3, 8 or 10of the isoalloxazine nucleus sensitized both strains. From ourdata, we conclude, that a) a cellular flavin controls the sensitivityof Neurospora crassa to light; b) that this flavin compoundis riboflavin; and c) that the active riboflavin is not proteinbound. ⁴Present address: Teikoku Women's University, Department ofHome Economics, 6-173 Touda-cho, Moriguchi-shi, Osaka, 570 Japan. (Received November 27, 1987; Accepted March 15, 1989)     

Circadian timekeeping in Neurospora crassa and Synechococcus elongatus

At first, the saprophytic eukaryote Neurospora crassa and the photosynthetic prokaryote Synechococcus elongatus may seem to have little in common. However, in both organisms a circadian clock organizes cellular biochemistry, and each organism lends itself to classical and molecular genetic investigations that have revealed a detailed picture of the molecular basis of circadian rhythmicity. In the present chapter, an overview of the molecular clockwork in each organism will be described, highlighting similarities, differences and some as yet unexplained phenomena.     

Altered Fatty Acid Distribution in Mutants of Neurospora crassa

Morphological mutants of Neurospora with decreased levels of reduced nicotinamide adenine dinucleotide phosphate (NADPH) and reduced nicotinamide ad enine dinucleotide (NADH) contained only 20% as much of a polyunsaturated fatty acid (linolenic acid) as the wild type in both the phospholipid and neutral lipid fractions. There was an excellent correlation between linolenic acid levels and morphological appearance as a function of total NADPH content, but no correlation with NADH content. The linolenic acid deficiency was balanced by a relative increase in the amounts of the less unsaturated fatty acids (oleic and linoleic acids), but the level of three other fatty acids did not appear to be changed. This accumulation of these two precursors suggests that the NADPH deficiency preferentially affected the final desaturation step, i.e., the conversion of linoleic to linolenic acid. The NADPH needed for this reaction in vivo was probably generated by the pentose phosphate shunt, since mutations affecting the shunt lead to the decreased levels of linolenic acid. It is not clear whether the changes in fatty acid distribution affect the morphogenesis of Neurospora, or if these changes are just part of the NADPH-deficiency syndrome.     

Circadian Rhythms of Nucleic Acid Metabolism in Neurospora crassa

Wild-type, band, and fluffy strains of Neurospora crassa exhibit circadian rhythms of ribonucleic acid and deoxyribonucleic acid content in the growth-front hyphae of cultures grown on a solid medium. There is also a rhythm of (3)H-uridine incorporation into the nucleic acids of the band strain. Maximum incorporation precedes the peaks of nucleic acid content which occur during conidiation. As cultures age, ribonucleic acid content decreases rapidly and deoxyribonucleic acid content decreases gradually in standing, shake, and bubble cultures. A reduction of ribonuclease activity with age is also noted in standing and shake cultures. The nucleic acid content, nuclease activity, and changes associated with age vary with the culture conditions.