Membrane Protein Differences Correlated with the Development of Mating Competence in Tetrahymena thermophila1

Initiation is the contact-independent phase of sexual conjugation which occurs when mature cells of Tetrahymena thermophila are shifted from growth medium to a low-salt starvation buffer. Immaturity, like high-salt starvation, restricts the ability of cells to conjugate; immature cells do not conjugate in either low- or high-salt buffers. Comparisons between sexually mature cells starved in initiation-restrictive and initiation-permissive buffers, and between immature and mature cells starved in an initiation-permissive buffer permitted the analysis of membrane protein expression correlated with mating competence. No polypeptides identified by lactoperoxidase-catalyzed iodination were found to be specific to mating-competent cells; however, several polypeptides not present in initiated cells were found to be common to the cell surfaces of immature and non-initiated cells which suggests that (1) initiation involves the removal of specific proteins from the cell surface, and (2) immaturity may be due to an inability to initiate.     

Germline and Somatic Transformation of Mating Tetrahymena Thermophila by Particle Bombardment

Mating Tetrahymena thermophila were bombarded with ribosomal DNA-coated particles at various times in development. Both macronuclear and micronuclear transformants were recovered. Optimal developmental stages for transformation occurred during meiosis for the micronucleus and during anlagen formation for the macronucleus. Evidence is given for transient retention of the introduced plasmid. Genetic and molecular tests confirmed that sexually heritable transformation was associated with integration at the homologous site in the recipient micronuclear chromosome.     

Genetic Instability in the Mating Type System of Tetrahymena pigmentosa

Selfing clones of Tetrahymena pigmentosa show several interesting genetic features, and provide some insight into the mechanisms of mating type (mt) determination. They differ significantly from those of Tetrahymena thermophila. They are distributed nonrandomly in crosses. Their rates of stabilization are highly variable, but most are much lower than those reported for T. thermophila. A number of subclones derived from nearly all the selfers have maintained stable mts in culture for several years. However, some subclones manifest persistent selfing, long after the calculated completion of allelic assortment for heterozygous loci. This phenomenon along with the perpetual maintenance of dominant mts in heterozygotes shows that phenotypic assortment is not involved in mt expression. In crosses, many selfers exhibit quantitative and qualitative aberrations in the transmission of alleles to the gametes; some of the micronuclear changes underlying these aberrations occur during vegetative growth. There are rare illegitimate appearances of dominant alleles in sexual progeny, and more common illegitimate appearances of the most recessive phenotype.--Various models to explain mt determination in this species are considered. One which might account for the troubling phenomena of the system consists of an active mat expression site, with "cassettes" at other sites specific for the different dominant alleles and capable of transposition to the expression site.     

Biochemical Approaches to Mating Type Expression in Tetrahymena thermophila1

Two-dimensional gel electrophoresis was used to identify the patterns of protein synthesis during initiation, and the patterns of membrane protein expression following initiation, in all of the mating types of the Tetrahymena thermophila B family. In addition, one-dimensional analysis was used to survey ¹²⁵I-Concanavalin A-binding proteins. Although a large number of proteins was identified by each technique, no variation among the mating types was observed.     

Induction of DNA polymerase in Tetrahymena pyriformis

A number of different treatments will induce DNA polymerase in Tetrahymena pyriformis. In the present paper we have studied the induction of DNA polymerase by the inhibitor of DNA synthesis methotrexate plus uridine (M+U) and UV irradiation (after incorporation of bromodeoxyuridine (BUdR) into DNA) in synchronized Tetrahymena populations. We have found that M+U must be present in the nuclear S-period in order to induce the polymerase, and that a dose of UV irradiation which is too low to induce DNA polymerase will do so if the damaging effect of the irradiation is enhanced by incorporation of BUdR into DNA.     

Traumatic Induction of Early Maturity in Tetrahymena

Exposure of conjugating pairs of Tetrahymena thermophila to high temperature (37°) during macronuclear development causes an abortion of many macronuclei, but it also often induces an early appearance of sexual maturity in clones completing macronuclear development. Lines become mature after about 15 cell divisions rather than after 50 or more cell divisions in untreated pairs. The phenotype resembles that associated with Em (early maturity) mutants but, because it is not transmitted to the progeny in the next generation, it must be considered a phenocopy. The hypothesis is developed that an early genotype-environment incompatibility, whether associated with an abnormal genotype or an unusual environment, activates a shunt mechanism permitting the organisms to undertake quickly an ordinarily forbidden sexual lottery.     

Induction of anti-actin drug resistance in Tetrahymena

Both cytochalasin D and latrunculin B reversibly inhibited Tetrahymena phagocytosis at concentrations similar to those effective in mammalian systems, even though ciliate actins are known to be highly divergent from mammalian actins. Overnight exposure to relatively low (0.25 microM) concentrations of latrunculin B induced resistance in Tetrahymena to the inhibitory effects of that drug, as well as cross-resistance to cytochalasin D. However, much higher (> 30 microM) concentrations of cytochalasin D were required for induction of cross-resistance to latrunculin B. Anti-actin drug resistance in Tetrahymena may involve a general multidrug resistance mechanism and/or specific feedback regulation of F-actin assembly and stability.     

Induction of a Metallothionein-like Protein in Tetrahymena pyriformis by Metal Ions

Trametes hirsuta produced cellulose-degrading enzymes when it was grown in a cellulosic medium such as Avicel or wheat bran. An endo-β-1,4-glucanase (ThEG) was purified from the culture filtrate, and the gene and the cDNA were isolated. The gene consisted of an open reading frame encoding 384 amino acids, interrupted by 11 introns. The whole sequence showed high homology with that of family 5 glycoside hydrolase. The properties of the recombinant enzyme (rEG) in Aspergillus oryzae were compared with those of the En-1 from Irpex lacteus, which showed the highest homology among all the endoglucanases reported. The rEG activity against Avicel was about 8 times higher than that of En-1 when based on CMC degradation. A remarkable structural difference between the two enzymes was the length of the linker connecting the cellulose-binding domain to the catalytic domain.     

Induction of thymidylate synthetase activity in Tetrahymena by cyclic guanosine monophosphate.

The induction of TMP synthetase activity in Tetrahymena pyriformis depended upon growth conditions. Enzymatic activity was low in cells grown in complex medium, and was high in cells grown in, or shifted to, defined medium. TMP synthetase activity rose 5 hours after the shift from complex to defined medium using uracil as the pyrimidine source. The time of induction was decreased to $\text{3}\text{1}\text{2}$ hours using dUMP as the pyrimidine source. cGMP or its dibutyryl derivative, but not cAMP, caused the induction of TMP synthetase activity in cells grown in complex medium. Caffeine, but not theophylline, mimicked the cGMP response. cAMP decreased both the cGMP and caffeine mediated increases in TMP synthetase activity. This is the first demonstration of an effect of cGMP on induction of an enzyme of pyrimidine metabolism in any cellular system.     

The Induction of Endocytosis in Starved Tetrahymena pyriformis

SYNOPSIS. The formation of digestive vacuoles by starved Tetrahymena pyriformis could be induced by mixtures of latex particles and a variety of potentially digestible solutes. Latex particles themselves had little effect in inducing vacuole formation. Protein, polypeptide, and RNA were highly effective inducers, while glutamate, amino acid mixtures, polysacharides, and glucose were moderately effective. Sodium-β-glycerophosphate had a slight effect and sodium acetate was ineffective. The possible stimulus to endocytosis is discussed. The endocytic response to inducers does not appear to be an all-or-none phenomenon and varies with the concentration of inducer. The stimulatory effect for protein-related inducers seems to be produced by a large number of stimulatory molecules acting upon a single cell and the magnitude of the response appears to be related to molecular size.     

Induction of DNA polymerase activity in irradiated Tetrahymena cells

Irradiation of Tetrahymena with sublethal doses of ultraviolet light or electrons provokes a several fold increase in the specific activity of the total DNA polymerase. The increase continues as long as the cell divisions are blocked after irradiation; thereafter the specific activity declines towards the level before irradiation. The induction of the enzyme is dependent on RNA- and protein synthesis.     

Isozymic Characterization of Three Mating Groups of the Tetrahymena pyriformis complex*

SYNOPSIS. Strains of 3 unnamed mating groups of the Tetrahymena pyriformis complex have been subjected to starch gel electrophoresis followed by staining the gels for the enzymes isocitrate dehydrogenase (NADP), tyrosine aminotransferase, and tetrazolium oxidase (superoxide dismutase). With respect to the electrophoretic mobilities of these enzyme systems, the mating groups referred to here as 5, 13 and 14 are very similar to Tetrahymena americanis (syngen 2), the most common North American species of the complex. Cultures in our collection labeled Tetrahymena cosmopolitans (formerly syngen 4) are either amicronucleate, with unique isozyme patterns, or micronucleate cells which mate with and have isozyme patterns similar to Tetrahymena canadensis (syngen 7). Immature progeny have been derived from crosses between the latter strains and T. canadensis recently collected in Colorado. The amicronucleate strains are now placed in the Tetrahymena sp. category, and we conclude that strains identifiable as T. cosmopolitanis are no longer available. The reliability of isozymes as characters in ciliate taxonomy was evaluated by comparing the present results for 3 enzymes in 15 groups of strains (syngens and phenosets) that had been compared in an earlier study. These enzyme systems gave correlation coefficients (r) of 0.75 or higher in the separate studies, and can be considered useful diagnostic traits. Other enzymes that were present at threshold levels of detectability or varied highly in concentration from species to species are too unreliable to be of diagnostic value. Some of the strains in the complex are so evolutionarily divergent at the molecular level that we have difficulty finding growth and electrophoretic conditions under which orthologous enzyme activities can be detected simultaneously for all the strains being compared.     

Induction of tubulin synthesis during cilia regeneration in growing Tetrahymena

Log growth Tetrahymena pyriformis GL were deciliated by means of a calcium pulse and allowed to regenerate their cilia in a non-nutrient recovery medium. Polyribosome profiles show only small amounts of polysomes up to 30 min after suspension in recovery medium. After this time the number of polysomes increases continuously as protein synthetic activity and motility are recovered. Labeling of whole cells with l-[³⁵S]methionine and comparison of the resulting electrophoretic patterns reveals a marked induction of tubulin synthesis as cilia regeneration proceeds. At its peak, tubulin accounts for 7–10% of the incorporated label but this peak occurs 35 min after the cells become greater than 90% motile and about 25 min after the cilia reach full length. These results are discussed with respect to the regulatory mechanism of tubulin induction and induction of tubulin synthesis in starved Tetrahymena.     

Mating type differentiation in Tetrahymena thermophila: Strong influence of delayed refeeding of conjugating pairs

Mating type differentiation in Tetrahymena thermophila is known to regularly involve stable hereditary alterations at a single chromosomal locus in the somatic (macro)nucleus. This differentiation is directionally affected by the temperature at which new macronuclei develop after fertilization. We now report large and predictable effects of delayed refeeding of conjugating pairs upon mating type differentiation, particularly among mat-2 homozygotes. The mating types whose frequency is affected the most are IV, VI, and VII, a set different from that most affected by temperature. We interpret our observations to reveal the existence of a second system which can participate in mating type differentiation, with different specificity from the system influenced by temperature under conditions of early refeeding of conjugating pairs. These observations enrich the phenomenology surrounding mating type differentiation in T thermophila and provide additional, easily controllable experimental conditions for the manipulation of mating type frequencies.     

Tip Transformation in Tetrahymena: A Morphogenetic Response to Interactions Between Mating Types*

SYNOPSIS. In Tetrahymena thermophila subline B, a morphogenic alteration of the anterior end of cells of mating types III and VII results from a cellular interaction which precedes and is a prerequisite for pairing. Cell pairing begins 1 h after starved cells of complementary mating type are mixed. The 1 h-long lag period is characterized by an actinomycin D-sensitive inductive interaction in the first 30 min, followed by a maturation period. Tip transformation begins during the maturation period and continues after pairing. Scanning electron microscopy of deciliated cells reveals ridges which form a chevron meeting in a midline seam between the oral apparatus and the anterior tip. During transformation, the seam broadens until the ridged surface is completely smooth. Melding of the ridges also occurs at the tip of the cell resulting in its blunted appearance. Cells of complementary mating types join in the region of this modified surface, which eventually becomes a specialized cell junction perforated by cytoplasmic bridges. Thus, pursuant to an inductive interaction the structure of the tip of cells is modified in anticipation of the pairing event. Rate of cell pairing might be limited by rate of tip transformation.