Two tissue culture media for production of lepidopteran cells and nuclear polyhedrosis viruses

Two media supporting the growth of several established lepidopteran cell lines in monolayer and suspension culture are described. The medium designated $\text{BML-TC}\text{10}$ was developed specifically as an inexpensive medium for production of cells of Spodoptera frugiperda and the homologous nuclear polyhedrosis virus (NPV) of this species. Simultaneously, a second medium was formulated in which the amino acid requirements were provided by enzymatic protein hydrolysates, one of which was termed $\text{BML-TC}\text{7A}$. Several cell lines could be adapted easily to this medium. $\text{BML-TC}\text{10}$ supported growth of S. frugiperda cells and production of the NPV's of S. frugiperda and Autographa californica. $\text{BML-TC}\text{7A}$ supported the growth of cells of S. frugiperda. Carpocapsa pomonella, Heliothis zea, and Trichoplusia ni. Cells of the latter produced the polyhedra of T. ni and A. californica NPV's in this medium.     

Brachymeria lasus: Culture in vitro of a chalcid insect parasite

The composition and formulation of an artificial medium and handling techniques are described for rearing the chalcid insect endoparasite, Brachymeria lasus (Walker) from the egg to adult stage under in vitro conditions. The medium was devoid of host materials, prepared aseptically, and contained 15% ($\text{w}\text{v}$) albumin, 1% amino acids, 4% glucose, and approximately 2.5% lipids, 0.3% inorganic salts, 0.01% B vitamins, and 0.2% lipogenic growth factors. Eggs were obtained by host dissection and developing larvae were reared in tissue culture plates. Adults were fecund.     

Conditions for protection of an allele in linear homogeneous stepping stone models

The one-dimensional linear homogeneous stepping stone migration structure is an important model in that it represents a short-range migration extreme for geographically structured populations and also serves as the underlying discretespace model for much of the work on continuous-space clines. We examine conditions for the protection of an allele under a stepping stone migration structure by using a recursive method based on Sturm sequences. Necessary and sufficient conditions for protection of an allele are found for a generalized step-cline selection gradient, which is the selection scheme used in much of the early cline work. Sufficient conditions for the protection of an allele are also found for (i) an advantageous patch at the stepping stone boundary which is followed by an arbitrary selection gradient, and for (ii) an advantageous patch embedded within an otherwise arbitrary selection gradient. We let m be the migration rate between neighboring demes. If within the advantageous patch $\text{W}{}_{\mathrm{Aa}}\text{W}{}_{\mathrm{aa}}\text{= 1 + s}$, then for (i) $\text{s ?}\text{m}\text{(1 ? m)}$ is sufficient to protect allele A, even if the patch consists of only a single deme, while for (ii) $\text{s ?}\text{2m}\text{(1 ? 2m)}$ guarantees that a single deme will protect A. If the advantageous patch consists of k demes, each with $\text{W}{}_{\mathrm{Aa}}\text{W}{}_{\mathrm{aa}}\text{= 1 + s,}\text{then}\text{s ? (}\text{π}{}^2\text{4}\text{)}\text{m}\text{k}{}^2$ is sufficient for protection of A in (i), while $\text{s ?}\text{π}{}^2\text{m}\text{k}{}^2$ is sufficient for protection of A in (ii). Sufficient conditions for a protected polymorphism are found, and a bound on the level of migration is determined, below which a protected polymorphism exists, as predicted from Karlin and McGregor's (1972. Theor. Pop. Biol.3, 186–209, 210–238) small parameter results. Finally, our patch swamping conditions (protection of an allele given a single advantageous patch) are compared to Nagylaki's (1975. Genetics80, 595–615) conditions for the existence of continuous-space clines under analogous selection schemes and are shown to be identical for the two specific cases examined. We also discuss extensions of some of the above results to circular stepping stone migration structures.     

Cytochrome P-450 and 18-oxygenase system from beef adrenocortical mitochondria - inhibitory effect of puromycin.

$\text{Trans}$-3-dehydro-D, L-ornithine and $\text{trans}$-1, 4-diamino-2-butene have been synthesized and shown to be potent competitive inhibitors of ornithine decarboxylase. The K_I′S for $\text{trans}$-3-dehydro-L-ornithine and $\text{trans}$-1, 4-diamino-2-butene are 2.2 and 2.0 μM respectively. Both analogs bind much more tightly to the enzyme than either ornithine or putrescine. Studies of chick embryo muscle cells in culture show results consistent with reversible inhibition of division and/or fusion by addition of $\text{trans}$-3-dehydro-D, L-ornithine to the culture medium.     

Macrophage migration inhibition by complement activators,migration inhibitory factor,and Lotus fucolectin: Evidence for common involvement of cell-associated esterase activity

Activators of the complement pathway were compared with migration inhibitory factor (MIF) and Lotus fucolectin, which mimics MIF, for their macrophage migration inhibitory (MMI) activity. Endotoxin (LPS), cobra venom factor (CVF), and zymosan, known complement (C3) activators, were found to produce dose-dependent MMI activity, similar to MIF, independent of requirements for nonadherent lymphocytes and serum complement. Comparable activity was observed by all migration inhibitors in the presence of freshly harvested unheated or heat-inactivated guinea pig serum as well as zymosan-adsorbed (C3-depleted) serum. Iscove's serum-free medium also promoted migration inhibition confirming a lack of requirement for serum complement in the reaction. Polymyxin B reversed MMI by LPS, but had no effect on the other inhibitors, indicating that the MMI activity of CVF, zymosan, MIF, and Lotus fucolectin was not primarily due to LPS contamination. Peritoneal macrophages (PM), depleted of nonadherent lymphocytes, responded as well as unpurified PM to the complement activators and MIF. ?-Amino-n-caproic acid (EACA), l-lysine, and tranexamic acid (TA), known inhibitors of the fibrinolytic activity of plasminogen activator (PA), were found to reverse migration inhibition of C3 activators, MIF, and Lotus fucolectin. In contrast bovine pancreatic trypsin inhibitor (BPTI) and soybean trypsin inhibitor (STI) had no effect on MMI activity. These results suggest a common mechanism for mediation of migration inhibition by complement activators and MIF which may involve activation of cell-associated complement to produce esterolytic end products capable of triggering the activation process.     

Transfer of cell-mediated immunity with cell-free leukocyte extracts: II. Demonstration of antigen-specific and nonspecific components

Transfer of cell-mediated immunity was achieved with dialyzable cell-free extracts from lymphoid cells of mice primed to the contact sensitizing agent, 2,4-dinitrofluorobenzene (DNFB). The biological activity of the extract (Transfer Factor, TF) was analyzed in vivo by the ear thickness assay and in vitro by the macrophage migration inhibition (MMI) test and lymphocyte transformation using the soluble analog, sodium 2,4-dinitrobenzenesulfonate. Consistently positive responses occurred 20 hr following a single intravenous injection of 5 × 10⁷ lymphocyte equivalents per recipient. The most potent source of TF (memory TF) was lymph node cells obtained 30 days after primary exposure to DNFB. By contrast TF prepared at the peak of the response to DNFB was less potent which was shown to be due to the presence in it of a suppressor factor. Memory TF elicited macrophage inhibition factor production in naive lymph node cells whereas positive responses were only obtained in the ear thickness and lymphocyte transformation assays provided recipients had undergone prior subliminal sensitization. Specificity of TF was tested using picryl chloride and oxazolone as control antigens. Results from the MMI and ear thickness assays were consistent with the presence in Transfer Factor of an antigen-specific component. Its effects, however, on the proliferative response to antigen lacked specificity and depended on prior sensitization of recipients, rather than donors, to the inducing antigen. The target of the specific component was considered to be an Ly-1⁺, Ia^?, $\text{Ly}\text{2}\text{3}{}^{\mathrm{?}}$ T cell since MIF production and in vivo delayed hypersensitivity are known to be mediated by a T cell bearing this phenotype. Taken together these findings emphasize the value of using a battery of tests of cell-mediated immune function when studying soluble mediators such as Transfer Factor and suggest that the current system is a valid experimental model for analysis of the Transfer Factor phenomenon.     

Alkaline and acid phosphatases of the marine diatoms Chaetoceros affinis var. willei (Gran) Hustedt and Skeletonema costatum (Grev.) Cleve

Alkaline phosphatase activity in cultures of the marine diatom Chaetoceros affinis var. willei (Gran) Hustedt was higher than in Skeletonema costatum (Grev.) Cleve. The enzyme activity was localized in coarse cell particles. Acid phosphatase activity was found in the cytoplasmic fraction. Induction of alkaline phosphatase depended on the $\text{N}\text{P}$ ratio in the culture medium. A $\text{N}\text{P}$ ratio > 40 in dilution/batch culture and > 30 in large scale batch culture, respectively, induced alkaline phosphatase.Cell phosphorus showed a critical value below which alkaline phosphatase was induced. Alkaline phosphatase in natural phytoplankton from the Trondheimsfjord is unlikely to occur except possibly in special situations.     

Precipitates and particulates cause proliferative activity of density-inhibited cultured cells by disturbing the diffusion boundary layer: An artefact superimposed upon an artefact?

Density-dependent inhibition of proliferation of cultured fibro-blast-like cells is based on depletion of essential medium factors from the diffusion boundary layer that is present close to the cell surface. Precipitates and particulates have been shown to cause proliferative activity when added to cultures of density-inhibited fibroblasts. $\text{It is proposed that precipitates and particulates cause proliferative activity in density-inhibited cultures by disturbing the diffusion boundary layer}$. The question of the suitability of density-inhibited fibrolasts for studies on initiation of cell replication is discussed as are other types of culture systems in which normal cells are proliferatively quiscent at low densities and under nutritionally replete conditions.     

Proteins shifting from the cytoplasm into the nuclei during early embryogenesis of Drosophila melanogaster

Monoclonal antibodies have been used to study the distribution of several proteins in cleavage and blastoderm stages of Drosophila melanogaster. These antigens are known to be associated with hnRNA-containing particles in tissue culture cells. Protein blotting shows that they are present in the embryo 1 hr after egg deposition. A redistribution from the cytoplasm into the somatic nuclei can be observed during developmental stage $\text{12}\text{13}$, one stage prior to the formation of the cellular blastoderm. Yolk nuclei become stained by these antibodies at about the same time. The shift into pole cell nuclei, however, occurs $\text{1}\text{1}\text{2}$ hr later, during the migration of these cells into the posterior midgut rudiment.     

An in vitro model for the study of collagen degradation during acute inflammation

Collagen sponges, labelled with fluorescein, were implanted under the back skin of sensitized rats. These elicited an acute inflammatory reaction with cellular invasion of the sponge and the development of a fibrous capsule at the periphery. After 4 days each sponge, together with the fibrous capsule, was excised and placed into tissue culture. Degradation of the collagen sponge by the invading cells was monitored from the release of soluble fluorescein peptides into the medium. The addition of foetal calf serum caused inhibition above 5% (v/v). Inhibitors of collagenase and neutral proteinases blocked the release of fluorescein peptides. Collagenolysis was also abolished or retarded by inhibitors of lysosomal cathepsins. The anti-inflammatory drug, dexamethasone, blocked all collagenolytic activity whereas indomethacin was without effect. The $\text{ex}$$\text{vivo}$ model offers the possibility for following the activity of the invading phagocytic cells and for examining the enzymatic mechanisms involved in collagenolysis using appropriate perturbation techniques.     

Side-specific analogues for the rat adipocyte sugar transport system

(1) 4,6-O-Ethylidene-d-glucose is a good inhibitor of adipocyte sugar transport from the external surface. Using radioactively labelled 4,6-O-methylidene-d-glucose we have shown that this compound is not taken up into cells by the hexose transporter but through a route which is insulin insensitive, d-glucose insensitive, temperature sensitive and which is slightly inhibited by phloretin. When efflux of 3-O-methyl-d-glucose is studied with 4,6-O-methylidene-d-glucose only present inside the cells then no detectable inhibition is observed indicating that this compound is a good side-specific analogue with a high affinity for only the external site of the hexose transporter. (2) Radioactively labelled alkyl-β-d-glucosides have been prepared. These also penetrate the adipocyte membrane by an insulin and d-glucose insensitive route. The half-times for equilibration with methyl-, n-propyl-, and $\text{n-}\text{butyl}\text{-β-}\text{d}\text{-}\text{glucosides}$ are 255, 9.45 and 3.3 min, respectively, indicating that the uptake rates are dependent upon the size of the alkyl group. (3) The glucosides show poor inhibition of 3-O-methyl-d-glucose transport when added to the external solution only. When cells are preincubated with $\text{n-}\text{propyl}\text{-β-}\text{d}\text{-}\text{glucoside}$ and $\text{n-}\text{butyl}\text{-β-}\text{d}\text{-}\text{glucoside}$ an increase in the amount of inhibition of 3-O-methyl-d-glucosez uptake is observed. This increase in inhibition correlates well with the glucoside uptake rates and indicates that availability of the glucosides at the internal surface of the transporter is required for inhibition. This has been confirmed by measuring 3-O-methyl-d-glucose exit in the presence of $\text{n-}\text{propyl}\text{-β-}\text{d}\text{-}\text{glucoside}$ at the internal surface only. Thus, $\text{n-}\text{propyl}\text{-β-}\text{d}\text{-}\text{glucoside}$ is a good side-specific analogue with high affinity only for the internal site of the hexose transporter. (4) $\text{n-}\text{Propyl}\text{-β-}\text{d}\text{-}\text{glucoside}$ inhibition of d-allose transport is fully reversible. If cells are washed after a preincubation with the analogue then the inhibition is lost. The $\text{n-}\text{propyl}\text{-β-}\text{d}\text{-}\text{glucoside}$ inhibition of d-allose transport is reduced competitively by 3-O-methyl-d-glucose. (5) 6-O-Propyl-d-galactose has low affinity for both internal and external sites.     

Induction and inhibition of meiotic maturation of follicle-enclosed porcine oocytes in vitro

Isolated porcine Graafian follicles which were explanted in vitro and maintained in organ culture were used as a test-system for the meiosis-inducing action of PMSG and hCG. The addition of either PMSG or hCG alone (10 or 20 IU/ml, respectively) to the culture medium was not effective, whereas the simultaneous administration of these hormones ($\text{15}\text{15}\text{IU/ml}$) induced resumption of meiosis in 90.3% ($\text{37}\text{41}$). The same hormone concentrations were used in a second series of experiments in which the inhibition and induction of meiosis of isolated oocytes were tested by transferring them into host follicles. In host follicles containing up to 12 foreign eggs, which were cultured in control media, meiosis was prevented in 86.0% of all oocytes ($\text{104}\text{121}$). By adding PMSG (15 IU/ml) simultaneously with hCG (15 IU/ml) to the medium, meiosis was induced in 95.0% of all oocytes ($\text{133}\text{140}$).The assumption is made that the signal initiating resumption of meiosis of the isolated and transferred oocytes is mediated by the follicular fluid, since intimate contact with the membrana granulosa of the host follicle was prevented by using a roller technique.     

Studies on purine transport and on purine content in vacuoles isolated from Saccharomyces cerevisiae

The transport of purine derivatives into vacuoles isolated from Saccharomyces cerevisiae was studied. Vacuoles which conserved their ability to take up purine compounds were prepared by a modification of the method of polybase-induced lysis of spheroplasts.Guanosine > inosine = hypoxanthine > adenosine were taken up with decreasing initial velocities, respectively; adenine was not transported.Guanosine and adenosine transporting systems were saturable, with apparent K_m values 0.63 mM and 0.15 mM respectively, while uptake rates of inosine and of hypoxanthine were linear functions of their concentrations.Adenosine transport in vacuoles appeared strongly dependent on the growth phase of the cell culture.The system transporting adenosine was further characterized by its pH dependency optimum of 7.1 and its sensitivity to inhibition by $\text{S-}\text{adenosyl-}\text{l}\text{-methionine}$.In the absence of adenosine in the external medium, [¹⁴C]adenosine did not flow out from preloaded vacuoles. However, in the presence of external adenosine, a very rapid efflux of radioactivity was observed, indicating an exchange mechanism for the observed adenosine transport in the vacuoles.In isolated vacuoles the only purine derivative accumulated was found to be $\text{S-}\text{adenosyl-}\text{l}\text{-homocysteine}$.     

Properties of a trypsin and chymotrypsin inhibitor secreted by larval Taenia pisiformis

Living metacestodes of Taenia pisiformis maintained in vitro discharge into the surrounding medium a protease inhibitor, which has been purified from the medium by affinity chromatography on bovine α-chymotrypsin immobilized to CNBr-activated Sepharose 4B. The purified inhibitor was shown to inactivate the hydrolysis of $\text{N-α-}\text{benzoyl}\text{-}\text{L}\text{-}\text{arginine}$ ethyl ester and $\text{N-}\text{benzoyl}\text{-}\text{L}\text{-}\text{tyrosine}$ ethyl ester, respectively, by trypsin and chymotrypsin of bovine, rabbit and dog origin, and also the hydrolysis of casein by both bovine trypsin and bovine α and β chymotrypsins, but it did not affect the enzymic activity of subtilisin, elastase, collagenase, pepsin, rennin and papain. The inhibitor withstood heating at 100°C for up to 30 min, was stable in the pH range of 1.5–8.0, was unaffected by 8 M-urea or 0.2 M-2-mercaptoethanol, and had a molecular weight of about 7000 as calculated from its gel chromatographic behaviour. The inhibitor specifically inhibits either trypsin or chymotrypsin with the formation of stable enzyme inhibitor complexes that are not dissociated by 4 M-KCl. Inhibition of trypsin and chymotrypsin is non-competitive and is linear with inhibitor concentration up to 70–80% inhibition. Inhibitory activities toward both enzymes are functions of the same binding site of the inhibitor molecule. Complex formation between the inhibitor and the enzymes is timedependent; it requires 3–4 min for completion.     

Erythrocyte Lii-Nao countertransport system Inhibition by N-ethylmaleimide probes for a conformational change of the transport system

Human erythrocytes were treated by a series of SH-reagents, including maleimides, iodo compounds, mercurials and oxidizing agents. Rates of Li efflux into Na-rich medium, Li leak and Li_i-Na_o countertransport were then determined. Of the 13 different reagents studied, only N-ethylmaleimide, iodoacetamide and iodoacetate inhibited selectively the countertransport activity. The effect of the various reagents indicates that the sensitive SH-groups of the countertransport system are not externally exposed. N-Ethylmaleimide was used to probe for changes elicited by substrate cations in Li_i-Na_o countertransport. In Na- and Li-free medium, inhibition of Li_i-Na_o countertransport by N-ethylmaleimide of 35% was reached within 2 s. In Na or Li medium, maximal inhibition was twice as great, but was attained much more slowly, within 10 min. Kinetic data and Hill plot analysis indicate the involvement of two classes of SH-groups: one expressed in the various media with and without substrate cations, and an additional one, which becomes specifically available to N-ethylmaleimide in the presence of external Na or Li. The affinity of Na to the site promoting inhibition by N-ethylmaleimide (apparent K_m  12 mM) is higher than the affinity of Na to its external countertransport site (apparent K_m  25 mM), as reported by Sarakadi, B., Alifimoff, J.K., Gunn, R.B. and Tosteson, D.C. (1978) J. Gen. Physiol. 72, 249–265). Reactivity of $\text{N-}\text{ethyl}\text{[}{}^{14}\text{C}\text{]}\text{maleimide}$ was not modified by the media tested. It is concluded that external Na and Li cause a conformational change in the protein(s) of the countertransport system in human erythrocytes.     

Estimation of mutation rates in cultured mammalian cells

The factors that affect reliable estimations of mutation rates (μ) in cultured mammalian somatic cell populations by fluctuation analysis are studied experimentally and statistically. We analyze the differential effect of the final cell population size in each culture (N_t) and the number of parallel cultures (C) on the variation in the rate estimates ($\text{μ}$) inferred from the P₀ method. The analysis can be made after the derivation of the variance of $\text{μ}$, which is a measure of variation of $\text{μ}$ for a given combination of N_t and C in a number of repeat experiments. The variance of $\text{μ}$ is inversely proportional to C and to the square of N_t. N_t determines the probability of occurrence of mutation in a cell culture. By influencing the size of P₀, N_t also determines whether a rate estimate is obtainable from the experiment. Since P_o is estimated from the fraction of cultures containing no mutation in a set of C cultures, C becomes a determining factor for the accuracy of $\text{μ}$. The rate estimated from $\text{P}\text{?}{}_0$ is biased, but the bias is in general 2 orders of magnitude smaller than $\text{μ}$. By the selection of an appropriate combination of N_t and C for the experiment, this bias can be reduced even further.Based on the notion of comparing two proportions, we propose a test statistic and have applied it to experimental results for a test of equality of mutation rates in different cell lines. This development places the comparison of mutation rates on a statistical basis.     

Differing responses of inbred rat strains in experimental autoimmune thyrioditis.

The CMI response in vitro and in vivo of 30 patients with a poor biologic response to infection with C. immitis was investigated. In patients with active pulmonary disease, skin reactivity to CDN was observed in $\text{7}\text{10}$, and to at least one of five other antigens in $\text{8}\text{10}$. In patients with the most extensive infection, disseminated disease, skin reactivity to CDN and to at least one of five other antigens was observed in only $\text{4}\text{8}$. In patients with inactive disease, skin reactivity to CDN and to at least one of five other antigens was observed in $\text{11}\text{12}$. Even when skin reactivity to CDN was present, MIF release and, more frequently, ³H-thymidine incorporation were not consistently stimulated by CDN. Maximal ³H-thymidine incorporation in response to PHA and CDN is delayed in 50% of the patients studied. The defect also may be present in patients with inactive disease; however, in two patients followed serially, lymphocyte function very slowly returned to normal. Rosette-forming cells were normal in $\text{18}\text{30}$.The frequency with which patients with coccidioidal disease demonstrate a defect in cell-mediated immunity raises unanswered questions about the mechanisms responsible for the defect and the role it may play in the biologic defense against invasion by this fungus.     

Alkaline phosphatase and maltase activity in the embryonic chick intestine in culture. Influence of thyroxine and hydrocortisone.

In strips of duodenum from 14-day chick embryos explanted into defined medium, alkaline phosphatase (ALP) activity accumulated in the tissue at a faster rate than in vivo for about 48 hr, but failed to increase thereafter. The addition of thyroxine (T4) to the medium at 10^?8M or less both enhanced the early accumulation and elicited a very large increase in ALP activity comparable to that normally occurring during the last 2 days in ovo. Activity with phenylphosphate (PhP) was more strongly affected than that with β-glycerophosphate (βGP), so that the high $\text{PhP}\text{β}\text{GP}$ ratio attained in vivo at 18 days was reached after 24 hr in T4-supplemented medium. Hydrocortisone (HC) evoked APL activity only slightly above that in unsupplemented medium and only during the first 48 hr in culture, but it precociously elevated $\text{PhP}\text{β}\text{GP}$ ratio to the normal maximum. In the presence of T4 or HC, maltase activity rose in explanted strips at the same rate as in the intact duodenum, but it lagged in unsupplemented medium. Assay of the medium revealed, however, that under all conditions of culture a large amount of both maltase and ALP activity had been released from the tissue. This effect was especially pronounced in the presence of T4, so that explants and medium together accumulated ALP and maltase equivalent to the high peaks of activity found in the intact duodenum at hatching. With 10^?8M T4, ALP activity began to rise above that of control explants after 8 hr, with accumulation in the medium beginning about 4 hr later. Combining 2 × 10^?6M HC with a range of T4 concentrations produced greater than additive effects, particularly with ALP, but did not lead to enhanced retention of either enzyme in the tissue strips. Prolactin, pentagastrin, and insulin were without effect alone, but the latter inhibited the effects of both T4 and HC.