A Comparative Study of the Changes in Root Growth, Induced by Coumarin, Auxin, Ethylene, Kinetin and Gibberellic Acid

The effect of coumarin, IAA, ethylene, kinetin and gibberellic acid on roots of maize and wheat was investigated. Sterile attached and detached roots and isolated elongation zones were used. In some experiments a semi-sterile procedure was followed. The effects of the different regulators separately or in various combinations together with coumarin were studied on the root growth with regard to division, elongation and swelling of the cells. The ethylene production in isolated elongation zones was measured after treatment with coumarin, IAA, PCIB, kinetin, colchicine and dinitrophenol. The results show the following: 1) Each substance produces a specific morphologic pattern. 2) Changes in polarity were demonstrated for auxin-induced swelling in cell divisions and cell expansion and for coumarin-induced swelling in cell divisions. Other cell expansion in swollen parts was due to cylindric cells increasing in width while retaining their cylindric form. 3) Coumarin-induced inhibition could not be counteracted by IAA, PCIB, carbon dioxide, kinetin, gibberellic acid or Cycocel. 4) The ethylene production in isolated elongation zones increases noticeably after kinetin treatment, less strongly after auxin treatment and least after coumarin treatment. The production of ethylene does not seem to be correlated with the morphogenetic effect of the different substances. 5) The isolated elongation zones reacted to a) IAA and kinetin with an increase in length in some cases and b) gibberellic acid with a reduction of their width. 6) The inhibitory effect of coumarin on the growth in length of the elongation zones was diminished by kinetin. The swelling produced by coumarin in these zones was reduced by gibberellic acid. The effects just mentioned of kinetin and gibberellic acid were considered as indirect ones. - From the present findings it was concluded that concomitant effects of auxin, ethylene, cytokinins and gibberellins are not obligatory for coumarin to exert its morphogenetic effects on root growth. In discussing the results some pitfalls in studies of growth reactions after application of hormones to roots containing meristem were emphasized.     

Effect of Purine and Pyrimidine Analogues on Growth and RNA Metabolism in the Soybean Hypocotyl-the Selective Action of 5-Fluorouracil

The effects of several base analogues and cycloheximide on RNA synthesis, protein synthesis, and cell elongation were studied in excised soybean hypocotyl. None of the pyrimidine analogues tested affected growth or protein synthesis; only 5-fluorouracil appreciably inhibited RNA synthesis. 8-Azaguanine and 6-methylpurine markedly inhibited RNA and protein synthesis and cell elongation. Cycloheximide effectively inhibited both cell elongation and protein synthesis.The results show that 5-fluorouracil selectively inhibited ribosomal and soluble RNA synthesis without affecting the synthesis of D-RNA. These results indicate that the requirement for RNA synthesis to support continued protein synthesis and cell elongation is restricted to the synthesis of D-RNA.5-Fluorouracil was incorporated into all classes of RNA in a form believed to be 5-fluorouridylic acid.Cycloheximide markedly inhibited the accumulation of ribosomal RNA, but the results indicate that CH did not inhibit, per se, the synthesis of ribosomal RNA. The accumulation of newly synthesized D-RNA was only slightly affected by cycloheximide. These results show that the inhibition of cell elongation by cycloheximide correlates with the inhibition of protein synthesis, but not with the effect on RNA metabolism.     

Inhibitors of poly (ADP-ribose) polymerase suppress lipopolysaccharide-induced nitrite formation in macrophages.

Stimulating bone marrow derived macrophages with LPS results in the induction of NO-synthase as measured by NO2- formation. Inhibitors of poly(ADP-ribose)polymerase, namely nicotinamide, 3-aminobenzamide and 3-methoxybenzamide, prevented NO2- formation in a dose dependent manner. Inhibition was most effective if the inhibitors were added at the same time as LPS. When added 10 h after exposure to LPS, a time at which expression of the enzyme had reached its maximum, no inhibition was observed. The inhibitors also blocked early events in activation such as protein and RNA-synthesis as well as DNA-synthesis. Thus prevention of NO2- formation may be related to inhibition of these events. Activation of macrophages by LPS was not accompanied by an increase but rather by a small decrease in ADP-ribosyltransferase activity. Whether this decrease plays a physiological role in activation needs further exploration.     

Protein Phosphorylation in Polysomes of Pumpkin Cotyledons after Coumarin Treatment

Abstract: The natural compound, coumarin, caused a change in protein pattern and influenced the phosphorylation status of some ribosome-associated proteins of pumpkin seedlings in vivo and in vitro. Low concentrations of coumarin stimulated ribosome-associated protein phosphorylation only in cotyledons but not in roots and stems. Two phosphoproteins whose phosphorylation state was influenced upon coumarin treatment could be isolated and characterized by their relative molecular weight of about 58 and 65 kDa and pl-values at 5.2 and 5.7, respectively. These phosphoproteins are not major constituents of small or large subunits of ribosomes. We did not find any influence of coumarin on phosphorylation of ribosomal proteins S6, LAO and LAI–3.     

Über die Wirkung von FdUrd auf den Nukleinsäure-Stoffwechsel von Zellen isolierter Gewebefragmente aus dem Thallus von Riella helicophylla

Summary In isolated thallus fragments of Riella dedifferentiation of mature cells takes place in a polar region. RNA-synthesis is stimulated first and then DNA-synthesis as well as nuclear and cell divisions in some of the cells. DNA-synthesis is blocked by 10^-5 M FdUrd while polarity of dedifferentiation disappears due to activation of RNA-synthesis in an increasing number of cells.The influence of FdUrd on RNA-synthesis in regenerating fragments has been investigated by determining incorporation of [¹⁴C₈]adenine-sulfate into nucleic acids and measuring the rate of turn-over of the latter. The nucleic acids were fractionated on columns of Sephadex G-150 and G-200 and subjected to electrophoresis on polyacrylamide gels.No differences in the rate of synthesis of the single species of RNA were found. Apparently, the synthetic capacity of the whole fragment is unchanged after treatment with FdUrd but the intercellular correlations which control the formation of meristematic centres are not evolved.After precipitation of the nucleic acids with ethanol the low molecular weight precursors in the supernatant were fractionated on Sephadex G-10 columns. After treatment with FdUrd the fraction of nucleotides has a higher rate of incorporation of [¹⁴C]adenine and a higher turn-over. It is assumed that the energy metabolism is changed when the cells are blocked at the beginning of the S-phase.

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Teil einer Dissertation der Fakultät für Mathematik und Naturwissenschaften der Technischen Universität Hannover.     

Nitrate Nutrition and Temperature Effects on Wheat: a Synthesis of Plant Growth and Nitrogen Uptake in Relation to Metabolic and Physiological Processes

Lawlor, D. W., Boyle, F. A., Keys, A. J., Kendall, A. C. andYoung, A. T. 1988. Nitrate nutrition and temperature effectson wheat: a synthesis of plant growth and nitrogen uptake inrelation to metabolic and physiological processes.—J.exp. Bot. 39: 329-343. Growth of spring wheat was measured in cool (13°C day/10°Cnight) or warm (23°C/18°C) temperatures, combined withlarge and small amounts of nitrate fertilizer. The rate of growthof dry matter was less at cool temperatures but total growthover the same period of development was slightly greater inthe cool than in the warm. Main-shoot and tiller leaves grewslower and, despite growing for a longer period, were shorterin the cool than in the warm. They had greater fresh and drymass and content of starch and fructosans per unit area. Coolconditions increased root dry mass, root to shoot ratio andnitrogen content in dry matter. Additional nitrate increasedleaf area of main shoots slightly but of tillers greatly; itincreased leaf and tiller dry matter and total plant dry mass.Additional nitrate decreased the proportion of dry matter inroots and in stems and the N content of dry matter in all plantparts. Regulation of growth by temperature, nitrate supply andthe rôle of photosynthesis and nitrogen uptake, is consideredin relation to the mechanisms of incorporation of carbon andnitrogen into biochemical constituents. It is concluded thattemperature regulates the rate of protein synthesis, which determinesplant growth rate. Nitrogen flux into the plant is not directlylinked to protein synthesis so that the content of NO^–₃and of amino acids is related both to growth and to conditionsgoverning NO^–₃ uptake and its reduction. When nitrogensupply is large, growth is limited by temperature, not NO^–₃.Inadequate nitrate supply decreases protein synthesis (and thereforegrowth) more than it decreases carbon assimilation, so thatorgans such as roots and stems increase in dry matter relativeto shoots and all tissues have smaller proportions of nitrogenin dry matter. Cool conditions, although decreasing the rateof protein synthesis, increase its duration and decrease thesize of leaves, so that the content of protein per unit leafarea is greater in cool than in warm grown leaves. Consequencesof changes in the balance of N and C supply and growth ratefor dry matter distribution in plants are discussed. Key words: Wheat, nitrate nutrition, temperature     

Cell elongation in the soybean root: The influence of inhibitors of RNA and protein biosynthesis

A possible requirement for RNA and protein synthesis duringcell elongation of intact seedling tissue was studied usingthe soybean seedling foot with the elongating zone being delineatedby India ink marks at 2 and 7 mm back of the root tip. In contrastto most excised plant tissues, there was marked net synthesisof RNA and protein during cell elongation of the intact root.AD and CH were potent inhibitors of cell elongation in the soybeanroot. CH essentially eliminated protein synthesis, whether measuredby net accumulation of protein or by ¹⁴C-leiicine incorporation,while completely inhibiting cell elongation after a short lag.AD, on the other hand, only partially inhibited protein synthesiswhile causing almost total inhibition of cell elongation aftera lag. The capacity of the tissue to synthesize protein in thepresence of AD was correlated with the maintenance of functionalpolyribosomes, thus suggestive that m-RNA associated with theregulation of cell elongation is more unstable (i.e., a shortermean life) than total root m-RNA. FU did not inhibit cell elongation,protein synthesis or the level of functional polyribosomes.The requirement for RNA synthesis during cell elongation ofthe seedling root, as in excised plant tissues, appears to berestricted to the AMPrich species of RNA presumed to be m-RNA. ¹This research was supported by NIH grant GM 10157. ²Purdue University AES paper No. 3359. ³Present address: Dept. of Botany, National Taiwan University,Taipei, Taiwan.     

Poly(ADP-ribose) synthesis and inhibition of DNA synthesis in Chinese hamster cells treated with methylating agents and thymidine

A possible role of poly(ADP-ribose) synthesis in modulating the response of V79 cells to DNA damage induced by N-methyl-N'-nitro-N-nitrosoguanidine (MNNG) and methyl methanesulfonate (MMS) was investigated. Inhibition of [3H]thymidine (dThd) incorporation into DNA and lowering of NAD+ levels in intact cells were employed as parameters of DNA-synthesis inhibition and poly(ADP-ribose) synthesis, respectively. Dose responses of these parameters were studied in cells 2 and 24 h after treatment with the methylating agents in medium with or without dThd. The initial inhibition of DNA synthesis was uniformly associated with stimulation of poly(ADP-ribose) synthesis whether the cells were treated with MNNG or MMS, incubated with or without 20 microM dThd which did not inhibit poly(ADP-ribose) synthesis, or incubated with 3 mM dThd which did inhibit the latter synthesis. By contrast, the DNA-synthesis inhibition detected 24 h after treatment with MNNG was not associated with poly(ADP-ribose) synthesis. These data suggest that (i) the mechanism of this later inhibition of DNA synthesis is different from that of the initial inhibition, (ii) DNA-synthesis inhibition does not stimulate poly(ADP-ribose) synthesis, and (iii) single-strand breaks, resulting from N-methylation of the DNA, stimulate poly(ADP-ribose) synthesis, which may produce the initial inhibition of DNA synthesis. The initial inhibition of DNA synthesis was not uniformly associated with mutagenesis and dThd facilitation of MNNG-induced cytotoxicity and mutagenesis. This indicates that O-methylation of DNA does not stimulate poly(ADP-ribose) synthesis. Our data suggest that, in V79 cells treated with methylating agents, poly(ADP-ribose) synthesis is stimulated by single-strand breaks, inhibits DNA synthesis, and thereby serves to allow time for repair of the DNA prior to replication.     

Synthesis,Antioxidant and Antiproliferative Evaluation,Molecular Docking and DFT Studies of Some Novel Coumarin and Fused Coumarin Derivatives

N′-[(4-Chloro-2-oxo-2H-chromen-3-yl)methylene]-2-cyanoacetohydrazide ( 3 ) was synthesized in excellent yield from the condensation of 4-Chloro-2-oxo-2H-chromene-3-carbaldehyde with cyanoacetohydrazide. Compound 3 was utilized as a building block to synthesize novel coumarin and heterocycle-fused coumarin derivatives. The chemical structures of all the new coumarin compounds were identified by spectral analyses. Some of the new coumarins compounds were screened in human cancer cell lines (HEPG-2, MCF-7, HCT-116 and PC-3) to learn about their cytotoxic effects in addition to the study of their DNA damage and antioxidant activity. Three of these compounds exhibited remarkable antioxidant and anti-proliferative activities. Moreover, they have the capability to protect DNA from damage induced by bleomycin. Molecular docking, DFT and molecular electrostatic potential studies were performed on the compounds in vitro.     

A comparison of cerebrosides, proteolipid proteins, and cholesterol as indices of myelin in the architecture of rat cerebrum

Abstract— —Serial frozen section sampling and microspectrophotometric assays were used to compare the fidelity of cerebrosides, proteolipid proteins (PLP) and cholesterol as indices of myelinated fibres in the somatosensory region of rat cerebrum. Cerebrosides (including sulphatides) were a satisfactory index regardless of the mode of expression. Per unit dry wt., they were lowest in layer II (4 per cent) and increased with the subpial depth to 16 percent in white matter. Elevations were seen at the locations of: the outer tangential plexus (1); the stripe of Kaes-Bechterew (2); the outer and inner stripes of Baillarger (3,4); and the inner tangential plexus (5), respectively. Expression in terms of residue protein, total lipid or DNA gave somewhat sharper profiles of the myeloarchitecture. PLP per unit dry wt. were lowest in layers I, II and III (2 per cent) and increased to 5·5 per cent in white matter. Peaks occurred near (3), (4) and (5). The PLP per cell and per unit residue protein rose six-fold, from the upper layers of cortex to white matter, and depicted the myeloarchitecture more faithfully. In general outline, PLP paralleled cerebrosides in distribution, in contrast with previous findings in human prefrontal cortex. Human cortex may contain more non-myelin PLP in the upper cortical layers owing to its greater wealth of neuropil and synapses. Cholesterol per unit dry weight was a poor index of the myeloarchitecture; it was lowest in layer II (5 per cent) and increased to 13-5 per cent in white matter without revealing the five horizontal bands of myelinated fibres. Expression of cholesterol in terms of total lipid or DNA improved its value as an index, but it was less satisfactory than cerebrosides.     

The effects of topping and plant population on dry matter synthesis and distribution in Brussels sprouts

The effects of topping at different dates, and of different plant populations on dry-matter production and distribution in Brussels sprouts were studied. Total dry-matter production per unit area was unaffected by either topping or density. Leaf area was decreased by topping, resulting in a temporary increase in net assimilation rate. Topping resulted in a redistribution of dry matter; that which would have formed new stem and leaf tissue was directed into sprout production. Increasing plant density did not affect the distribution of dry matter but increased the number of smaller sprouts. The apparent optimum plant spacing in this series was 21×21 in (53×53 cm). At maturity assimilation approximately balances respiration.     

Coumarin inhibitors of gyrase B with N-propargyloxy-carbamate as an effective pyrrole bioisostere

The synthesis and biological profile in vitro of a series of coumarin inhibitors of gyrase B bearing a N-propargyloxycarbamate at C-3' of noviose is presented. Replacement of the 5-methylpyrrole-2-carboxylate of coumarin drugs with an N-propargyloxycarbamate bioisostere leads to analogues with improved antibacterial activity. Analysis of crystal structures of coumarin antibiotics with the 24 kDa N-terminal domain of the gyrase B protein provides a rational for the excellent inhibitory potency of C-3' N-alkoxycarbamates.     

Effects of Glomus fasciculatum and isolated rhizosphere microorganisms on growth and phosphate uptake of Plantago major ssp. pleiosperma

An experiment was set up in order to study 1) the relationship between net P uptake and dry matter production in mycorrhizal and non-mycorrhizal plants and 2) the effects of isolated rhizosphere bacteria and fungi on net P uptake and growth of P. major ssp. pleiosperma. A similar relationship between net P uptake and dry matter production was found for both mycorrhizal and non-mycorrhizal plants, although the regression lines differed in intercept.Compared to non-inoculated treatments, inoculation with bacteria slightly decreased dry matter production and P uptake of P. major, whereas inoculation with fungi or bacteria + fungi showed no effect. The results are discussed in terms of competition for available P and host photosynthates between host plant and rhizosphere microorganisms.     

Regulation of protein accumulation in cultured cells.

1. A technique is described whereby protein synthesis, protein breakdown and net protein accumulation are measured separately in monolayer cultures of mammalian cells. All rates are expressed as microgram of protein per 18 h incubation. 2. Under most incubation conditions with either L6 rat myoblasts or T47D human breast carcinoma cells the rates of protein accumulation, determined directly, agreed with the rates obtained by subtracting protein breakdown from protein synthesis. 3. Foetal calf serum, human and bovine colostrum, human milk and insulin increased protein accumulation in both cell lines, mainly as a consequence of effects on protein synthesis. 4. NH4Cl, in addition to inhibiting protein breakdown in both cell lines in the presence and in the absence of serum, stimulated protein synthesis in L6 myoblasts. 5. Leupeptin slightly inhibited protein breakdown without affecting protein-synthesis rates. 6. Cycloheximide almost completely inhibited protein synthesis, but restricted the net loss of cell proteins under most conditions because protein-breakdown rates were also decreased. 7. The assumptions, limitations and potential application of this technique for evaluating changes in protein turnover are described.     

Ribonucleic acid synthesis in rabbit erythroid cells.

Kinetic studies on the synthesis of RNA in mature bone-marrow erythroid cells from rabbits were made by measuring the incorporation of [2-3H]adenosine into the ATP pool and RNA over periods up to 8h. By use of equations to fit the pool specific radioactivity and an equation using the same type of pool to generate the rate of linear DNA synthesis, good agreement between the pool parameters is found, provided that the ATP pool is measured in whole cell extracts, and assuming that the dATP and ATP pools equilibrate rapidly. RNA-synthesis rates were measured by using curve fits to equations developed by using the pool specific-radioactivity curves. The rate of synthesis of poly(A)-containing RNA varied in three experiments from 90 to 220mol/min per cell, with half-life of nuclear processing of 12-22 min with a mean of 16 min. Ribosomal RNA is synthesized at a rate of 70-200 mol/min per cell with an average half-life of nuclear processing of 37 min for the 18S RNA and 214 min for the 28S RNA. When the stable rRNA components are subtracted from the nRNA synthesis, the rate of nRNA synthesis is between 2 and 6fg/min per cell with an average half-life of degradation of 27 min. The rate of synthesis of poly(A)-containing RNA is 1.5-3.5% of the RNA-synthesis rates. These rates are compared with the RNA-synthesis rates found in L cells and concentrations of globin mRNA found in various erythroid-cell preparations.     

Coumarin inhibits the growth of carrot (Daucus carota L. cv. Saint Valery) cells in suspension culture

We used a carrot (Daucus carota L. cv. Saint Valery) cell suspension culture as a simplified model system to study the effects of the allelochemical compound coumarin (1,2 benzopyrone) on cell growth and utilisation of exogenous nitrate, ammonium and carbohydrates. Exposure to micromolar levels of coumarin caused severe inhibition of cell growth starting from the second day of culture onwards. At the same time, the presence of 50 mumol/L coumarin caused accumulation of free amino acids and of ammonium in the cultured cells, and stimulated their glutamine synthetase, glutamate dehydrogenase, glucose-6-phosphate dehydrogenase and phosphoenolpyruvate carboxylase activities. Malate dehydrogenase, on the other hand, was inhibited under the same conditions. These effects were interpreted in terms of the stimulation of protein catabolism and/or interference with protein biosynthesis induced by coumarin. This could have led to a series of compensatory changes in the activities of enzymes linking nitrogen and carbon metabolism. Because coumarin seemed to abolish the exponential phase and to accelerate the onset of the stationary phase of cell growth, we hypothesise that such allelochemical compounds may act in nature as an inhibitor of the cell cycle and/or as a senescence-promoting substance.     

Coumarin effects on Glycine max hypocotyl explants

Coumarin induced root formation and stimulated fresh weight production in hypocotyl explants of Glycine max L. cultured in vitro. All stimulatory effects caused by coumarin were induced within a relatively narrow range of concentrations between 1–500 μM, yielding optimum dose response curves. When coumarin was combined with kinetin fresh weight increased considerably, at optimum concentrations to a level almost as high as that obtained with NAA (10 μM) and kinetin (10 μM). Root formation was almost completely inhibited when kinetin was added in combination with coumarin. NAA + coumarin had small stimulatory effects on fresh weight. but were inhibitory in root formation. The frequency of rooting per explant, texture and pigmentation were also affected by different treatments.     

Early Inhibition of Cellular DNA Synthesis by High Multiplicities of Infectious and UV-Inactivated Reovirus

Inhibition of cellular DNA synthesis began 6 to 8 h after reovirus infection at a multiplicity of infection of 10 PFU per cell. However, as the multiplicity of infection was increased to a maximum of 10³ PFU/cell, inhibition of DNA synthesis began earlier after infection (2-4 h postinfection), and the initial rate of inhibition increased. The enhanced inhibition of DNA replication at high virus multiplicities appeared to be selective since RNA synthesis was not detectably altered as late as 9 h postinfection and inhibition of protein synthesis did not begin until 7 to 9 h after infection. Early inhibition of DNA synthesis did not appear to be related to changes in thymidine pool characteristics, thymidine kinase activity, or detectable degradation of cellular DNA. Even though the particle-to-PFU ratio was increased by ultraviolet light inactivation of virus, the ability to induce early inhibition of DNA synthesis was not diminished.     

Fermentation of peptides and amino acids by a monensin-sensitive ruminal Peptostreptococcus

A monensin-sensitive ruminal peptostreptococcus was able to grow rapidly (growth rate of 0.5/h) on an enzymatic hydrolysate of casein, but less than 23% of the amino acid nitrogen was ever utilized. When an acid hydrolysate was substituted for the enzymatic digest, more than 31% of the nitrogen was converted to ammonia and cell protein. Coculture experiments and synergisms with peptide-degrading strains of Bacteroides ruminicola and Streptococcus bovis indicated that the peptostreptococcus was unable to transport certain peptides or hydrolyze them extracellularly. Leucine, serine, phenylalanine, threonine, and glutamine were deaminated at rates of 349, 258, 102, 95, and 91 nmol/mg of protein per min, respectively. Deamination rates for some other amino acids were increased when the amino acids were provided as pairs of oxidized and reduced amino acids (Stickland reactions), but these rates were still less than 80 nmol/mg of protein per min. In continuous culture (dilution rate of 0.1/h), bacterial dry matter and ammonia production decreased dramatically at a pH of less than 6.0. When dilution rates were increased from 0.08 to 0.32/h (pH 7.0), ammonia production increased while production of bacterial dry matter and protein decreased. These rather peculiar kinetics resulted in a slightly negative estimate of maintenance energy and could not be explained by a change in fermentation products. Approximately 80% of the cell dry matter was protein. When corrections were made for cell composition, the yield of ATP was higher than the theoretical maximum value. It is possible that mechanisms other than substrate-level phosphorylation contributed to the energetics of growth.     

Relationship between cellular autolytic activity, peptidoglycan synthesis, septation, and the cell cycle in synchronized populations of Streptococcus faecium.

Synchronized, slowly growing (TD = 70 to 80 min) cultures were used to study several wall-associated parameters during the cell cycle: rate of peptidoglycan synthesis, septation, and cellular autolytic activity. The rate of peptidoglycan synthesis per cell declined during most of the period of chromosome replication (C), but increased during the latter part of C and into the period between chromosome termination and cell division (D). An increase in cellular septation was correlated with the increased rate of peptidoglycan synthesis. Cellular autolytic capacity increased during the early portion of C, reached a maximum late in C or early in D, and declined during D. Inhibition of DNA synthesis during C prevented the decline in autolytic capacity at the end of the cell cycle, caused a slight reduction in the rate of peptidoglycan synthesis, delayed but did not prevent septation, and prevented the impending cell division by inhibiting cell separation. Inhibition of DNA synthesis during D did not prevent the increase in autolytic capacity during the next C phase, but, once again, prevented the decline at the end of the subsequent cycle. Thus, increased autolytic capacity at the beginning of the cell cycle did not seem to be related to chromosome initiation, whereas decreased autolytic capacity at the end of the cell cycle seemed to be related to chromosome termination. The data presented are consistent with the role of autolytic enzyme activity in the previously proposed model for cell division of S. faecium (G.D. Shockman et al., Ann. N.Y Acad. Sci. 235:161-197, 1974).