Preleptotene chromosome contraction in Lilium longiflorum “Croft”

A period of chromosome contraction between premeiotic interphase and leptotene was regularly observed in three samples of Lilium longiflorum Croft. Extensive preleptotene chromosome contraction was also observed in L. longiflorum Ace and in the Lilium hybrid Enchantment. Although the stage resembles late mitotic prophase, microsporocytes never develop to metaphase, but despiralize to leptotene, and regular alignment, pairing and chiasma formation follow. As preleptotene chromosome contraction is discovered in an increasing number of organisms it becomes less likely that it represents a true reversion to mitosis. However its absence in many organisms and its extreme variability in others do not support the concept of preleptotene chromosome contraction as a regular meiotic stage. It is suggested that the line of demarcation between mitosis and meiosis is often imprecise, and meiocytes may fluctuate to some extent between these states before a final transition to meiosis is made. The occurrence and extent of this fluctuation may possibly be related to some externally produced substances required for the orderly development of meiotic prophase.     

Evidence on the time of chromosome pairing from the preleptotene spiral stage in Lilium longiflorum “Croft”

A period of chromosome spiralization and contraction was observed between premeiotic interphase and leptotene in Lilium longiflorum Croft. There was variation in the extent of preleptotene spiralization and contraction of chromosomes among microsporocytes, anthers and buds. The chromosomes sometimes contracted sufficiently to be visible as separate entities. It could then be determined that the chromosomes were single and entirely separate; synapsis and crossing-over had not yet occurred. Furthermore there was no evidence of alignment or association of homologues during the preleptotene contraction period; the chromosomes appeared to be distributed at random. The chromosomes subsequently elongated into the leptotene stage. Wherever they were visible separately the chromosomes were single in early leptotene. These observations support the classical view that synapsis of homologous chromosomes takes place during zygotene, followed by crossing-over at pachytene.It is a pleasure to dedicate this paper to Dr. Sally Hughes-Schrader on the occasion of her seventy-fifth birthday.     

A test of distributive pairing in Zea mays

Zea mays plants containing two extra chromosomes were analyzed to determine if distributive pairing takes place in maize. No interaction between two univalent chromosomes generated in such plants could be detected at diakinesis or metaphase I. The chromosome disjunction in such plants was random at anaphase I. Furthermore, it was found that two chromosomes which are found as univalents in essentially 100 percent of the meiotic cells assorted randomly to the progeny. These experiments duplicated as closely as possible certain of Grell's (1962) experiments on distributive pairing. The author could detect no evidence for distributive pairing in maize. It was concluded that distributive pairing either does not occur in maize or that it occurs with a far lower efficiency than it does in Drosophila melanogaster females. Speculations on the reasons for these differences are included.Research supported in part by a grant (GM82-08) from the National Institutes of Health, U. S. Public Health Service.     

Development of the synaptonemal complex and the “recombination nodules” during meiotic prophase in the seven bivalents of the fungus Sordaria macrospora Auersw

Complete reconstruction of seven leptotene, six zygotene, three pachytene and three diplotene nuclei has permitted to follow the pairing process in the Ascomycete Sordaria macrospora. The seven bivalents in Sordaria can be identified by their length. The lateral components of the synaptonemal complexes (SC) are formed just after karyogamy but are discontinuous at early leptotene. Their ends are evenly distributed on the nuclear envelope. The homologous chromosomes alignment occurs at late leptotene before SC formation. The precise pairing starts when a distance of 200–300 nm is reached. Each bivalent has several independent central component initiation sites with preferentially pairing starting near the nuclear envelope. These sites are located in a constant position along the different bivalents in the 6 observed nuclei. The seven bivalents are not synchronous either in the process of alignment or in SC formation: the small chromosomes are paired first. At pachytene the SC is completed in each of the 7 bivalents. Six bivalents have one fixed and one randomly attached telomeres. The fixed end of the nucleolar organizer is the nucleolus anchored end. At diffuse stage and diplotene, only small stretches of the SC are preserved. The lateral components increase in length is approximately 34% between leptotene and pachytene. Their lengths remain constant during pachytene. From zygotene to diplotene the central components contain local thickenings (nodules). At late zygotene and pachytene each bivalent has 1 to 4 nodules and the location of at least one is constant. The total number of nodules remains constant from pachytene to diplotene and is equal to the mean total number of chiasmata. The observations provide additional insight into meiotic processes such as chromosome movements, initiation and development of the pairing sites during zygotene, the existence of fixed telomeres, the variations in SC length. The correspondence between nodules and chiasmata are discussed.     

Transition from somatic to meiotic pairing and progressional changes of the synaptonemal complex in spermatocytes of Aedes aegypti

Aedes aegypti spermatocytes were reconstructed from electron micrographs. The species has tight somatic pairing of the chromosomes, and there are therefore no classical leptotene and zygotene stages, but rather a gradual transition from somatic pairing to meiotic pairing (= pachytene). The term prepachytene has been used for the transitory stage. The first visible sign of impending meiosis was a reorganization of the chromatin, which resulted in the formation of spaces (synaptic spaces) in the chromatin, about the width of the synaptonemal complexes (SCs). Diffuse material, possibly precursor material for the SC, was present in the spaces. Later short pieces of complex were formed throughout the nucleus. Late prepachytene, pachytene, and diplotene complexes were reconstructed. Each chromosome occupied a separate region of the nucleus. The complexes became progressively shorter from prepachytene (maximum complement length 289 m) to diplotene (175 m). The thickness of the SCs increased from prepachytene to pachytene and probably decreased again during diplotene. At the beginning of diplotene the lateral elements (LEs) separated, and the single LEs became two to three times thicker than the LEs of the SC. The centromeres were at all stages attached to the nuclear membrane, whereas the telomeres were free in the nucleoplasm during pachytene and diplotene. A heterochromatic marker was present on chromosome 1 near the sex determining locus, and a diffuse marker on chromosome 3 near the nucleolus organizer region. After breakdown of the complexes, polycomplexes were present in the nucleus.     

Involvement of protein kinase A and casein kinase II in thein vivo protein kinase activities in prophase arrested Xenopus oocytes

In vivo casein phosphorylation was analysed in Xenopus full-grown oocytes arrested in the prophase of the meiotic cell division. The phosphorylation was inhibited by the protein kinase inhibitor (PKI) and also by heparin (3 g/ml; final concentration). casein phosphorylation was increased by spermine (2 mM). Therefore, protein kinase A and casein kinase II are both activein vivo in full-grown oocytes and may be involved in the prophase arrest of meiotic cell division.     

A test of distributive pairing in Zea mays utilizing doubly monosomic plants

Summary The v _x1 deficiency in Zea mays induces chromosomal nondisjunction during the megagametophyte divisions after meiosis producing large numbers of monosomes, trisomes, double monosomes, double trisomes, and even triple monosomes. In this study, microsporogenesis in six doubly monosomic combinations was analyzed. Double monosomes in a diploid organism provide the ideal material to determine if there is an interaction between two nonhomologous univalent chromosomes because two nonhomologous chromosomes lacking partners are present in each meiotic cell.At diakinesis and metaphase I, the two nonhomologous monosomic chromosomes were infrequently paired (3.76% and 2.18% respectively). These estimates are the upper estimates of pairing of nonhomologous monosomic chromosomes and probably represent an overestimate of these values because cells with any connections between the monosomic chromosomes were scored as having nine pairs and similar connections are not infrequently observed between two bivalents.The transmission of two nonhomologous unpaired chromosomes was deduced by studying the progeny of maize plants hyperploid for two chromosomes (a B⁴ and Wd ring). The two nonhomologous univalents disjoined randomly.Since no evidence for an interaction between nonhomologous univalent chromosomes which leads to their non-random disjunction to opposite poles was found in this study, these data confirm my earlier conclusion (Weber, 1966, 1969) that distributive pairing does not occur in maize (and probably most other plants) or that it occurs with a much lower efficiency than in Drosophila females. The frequent pairing between nonhomologous chromosomes at diakinesis and metaphase I and the non-random distribution at anaphase I in doubly trisomic maize plants reported by Michel and Burnham (1969) was found neither in my earlier studies (Weber, 1966, 1969) nor in the present study. The current study is far more sensitive than any of the previous studies because two nonhomologous chromosomes lacking pairing partners are found in every cell of a doubly monosomic plant.Research supported in part by U.S. Atomic Energy Commission Contract AT(11-1)-2121. Tech. Report No. COO-2121-10. This paper is dedicated to Professor Marcus M. Rhoades on the occasion of his 70th birthday. His guidance and help will be cherished throughout my lifetime.     

Meiosis readiness in Lilium longiflorum “Croft”

It is proposed that anthers of Lilium longiflorum Croft approaching the end of premeiotic mitosis reach a state described as meiosis readiness after which cells in premeiotic prophase are unable to complete a mitotic division but despiralize to interphase and enter a meiotic division. Many of the laggard premeiotic cells begin despiralization before reaching an extremely contracted state of late prophase. Premeiotic despiralization is not, therefore, attributed to a deficiency in metaphase but to an inability of these cells to complete prophase. Premeiotic despiralization appears to be preceded by a slowing-down of prophase development. There is variation among anthers and anther regions in the onset of prophase retardation and meiosis readiness. It is suggested that meiosis readiness depends upon a gradual accumulation of meiosis-inducing substances in the cytoplasm of the premeiotic cells. It has not been determined whether the cells that undergo premeiotic despiralization give rise to the giant microsporocytes with shattered chromosomes observed at late prophase of meiosis.     

Intranuclear fibrillar material in cereal pollen mother cells

Ultrastructural studies of cereal anthers found intranuclear bundles of microfilaments in pollen mother cells (PMCs) but not elsewhere. The ultrastructure, distribution, and behaviour of this fibrillar material (FM) are described. FM was seen in all 19 genotypes studied comprising Aegilops, Triticum, Secale, Hordeum and Avena species, which together included haploid, diploid and allo-and autopolyploid, and natural and synthetic polyploid examples. Detailed studies in diploid S. cereale, and hexaploid T. aestivum and Triticale showed that FM was present in PMC nuclei during premeiotic interphase, leptotene and zygotene but not at pachytene and later meiotic stages. Moreover, it was most abundant at late premeiotic interphase in T. aestivum, and at leptotene in S. cereale and Triticale, when it occurred in up to 100% of sampled PMC nuclei in an anther. Although FM and synaptonemal complex (SC) occurred together in some PMC nuclei at later stages, FM was present long before SC, and reached its peak of abundance before SC did. Bundles of FM often formed links at their ends between either two masses of chromatin, or more rarely, between chromatin and the nuclear membrane. Individual bundles of FM varied in length but showed roughly similar ranges of lengths and widths in these three species. They were up to about 0.2 m in diameter and about 3 m in length, equivalent to about 20% of the maximum diameter of the nuclei containing them. Reconstructions of PMC nuclei indicated that FM was never associated with centromeres but was sometimes, and perhaps usually, associated with telomeric or sub-telomeric chromosome segments.The function of FM is unknown but its possible role is discussed in relation to (1) previously described intranuclear inclusions in meiocytes and (2) the cytogenetics and developmental behaviour of meiotic nuclei in the wheat comparium. As FM was a constant and characteristic structural component of PMC nuclei, its presence is probably of functional significance to the meiotic process. If so, it may function before, and over greater distances, than SC in establishing or maintaining the coorientation of chromosomes prerequisite for normal chromosome pairing. As FM was most abundant at stages when major chromosome movements occur, yet its distribution was non-centromeric, it is suggested that it may function in the attachment and movement of telomeres at the nuclear membrane formed after premeiotic mitosis. The possibility that a bundle of FM normally links corresponding sites on two homologues is considered.     

Histone synthesis during meiotic prophase in Lilium

Anthers of Lilium candidum L. were cultivated on artificial media containing labelled amino acids. Histones were isolated from meiocytes and fractionated by the use of polyacrylamide gel electrophoresis (PAGE). Total histone synthesis was found not to terminate at the end of premeiotic interphase but to continue until at least zygotene. However, the rate of synthesis was reduced during prophase I compared to interphase. Separate fractions were synthesized asynchronously during the period from late interphase to zygotene. Tissue specific histone of meiosis (FM) was synthesized during late interphase and leptotene.Dedicated to Professor A. A. Prokofieva-Belgovskaia on the occasion of the seventieth anniversary of her birthday.     

Between-family variation in sex ratio in the Trinidad (T-30) strain of Aedes aegypti (L.) indicating differences in sensitivity to the meiotic drive gene M D

Sex ratio in the Trinidad (T-30) strain of Aedes aegypti has remained constant at around 43% during seventeen years of laboratory culture. The divergence from 50% is due to meiotic drive by the M ^D gene on the Y chromosome. The driving Y chromosome gives a much more distorted sex ratio (mean = 5.7%) when coupled with the highly sensitive X chromosomes from strain 64. This was demonstrated in all of 98 families tested, indicating that all or most of the Y chromosomes in T-30 carry the M ^D gene. Consequently the low level of sex ratio distortion in T-30 must be due to resistance to M ^D.Crosses made within T-30 demonstrated wide differences in sex ratio between families, depending on the sensitivity of the male parent's X chromosome to M ^D. However, sex ratios were not continuously variable but fell within fairly discrete categories. Thus, X chromosomes could be classified according to the modal sex ratios associated with them: m ^s3 (12.5%), m ^s2 (32.5%), m ^s1 (40%), m ^r1 (47.5%) m ^r2 (57.5%).The different sex ratio categories were more discrete in the families of sib matings than from random matings, suggesting the possibility of background modification of what is essentially a balanced polymorphism. Evidence is presented suggesting that the polymorphism could be due to interaction at two loci. A further X variant, m ^s4 (<10%) characterised strain 64 but was absent from T-30.A comparison of fertility between the different sex ratio categories in T-30 established that sex ratio distortion was not caused by differential mortality after fertilisation.     

Cyto-morphological studies op some species and hybrids in the Eu-Sorghums

Summary Important morphological features such as plant height, leaf size and number of leaves, shape of the panicle and sessile spikelets, staminate condition of the pedicellate florets, nature of lemma, colour of the stigmatic surface and seeds etc., were studied in 8 Sorghum species and 10 F₁ hybrids between them. Based on the data, interrelationship amongst the species are discussed.Pachytene pairing was complete and apparently normal, followed by regular meiosis at later stages resulting in high pollen stainability and good seed setting in all the parental species except the male sterile Kafir. Studies on the pairing properties of the differentially stained regions showed that synapsis starts from the proximal to the distal end and separation of the split chromosomes starts from the distal to the proximal.The interspecific hybrids studied are classified into four types based on pachytene pairing and pollen sterility. 1. normal pairing accompanied by high pollen fertility, 2. normal pairing accompanied by partial pollen sterility. 3. irregularities in the pachytene pairing followed by partial pollen sterility and 4. irregularities in the pachytene pairing accompanied by normal pollen fertility. Suitable explanations are advanced to explain the meiotic aberrations noted in some of the hybrids under study.Cytogenetical mechanisms underlying species differentiation in the Eu-Sorghum species are discussed.     

Non-reciprocal gonadal dysgenesis in hybrids of the chironomid midge Chironomus thummi

In male hybrids of the cross Chironomus thummi thummi (stock Hl) x Ch. th. piger (stock E) , but not the reciprocal cross, rudimentary testes develop at a growth temperature of 21 ° C. Within the dysgenic testes of these hybrids a number of abnormalities are observed which are restricted to the germ line. Approximately 60% of the hybrid males show allocyclic chromosome behaviour in spermatogonia and spermatocyte I nuclei. Within these nuclei two groups of four chromosomes are formed which differ from one another in their state of condensation. Each chromosome group consists of three long and one short chromosome. In cases where allocycly is very pronounced, the chromosomes of both groups disintegrate into numerous unequally sized fragments at meiotic prometaphase I, and gametes are not produced. In individuals, in which the allocycly is less pronounced or absent the nuclear divisions appear to be normal but chromosome and chromatid aberrations are frequent, and the number of viable sperm is reduced. In these males, the chiasma frequency is also decreased more than 12-fold in comparison with the reciprocal, unaffected piger x thummi hybrids.     

Acclimation of the Sea Cucumber Apostichopus japonicus to Decreased Salinity at the Blastula and Gastrula Stages: Its Effect on the Desalination Resistance of Larvae at Subsequent Stages of Development

Apostichopus (= Stichopus) japonicus blastulae and gastrulae were acclimated for 18 h to salinities of 32 (control), 24 and 22 (the lower limit of the range of tolerance), and 20 (below the range of tolerance). Acclimation to 20 resulted in the appearance of teratic larvae, most of which subsequently died. Acclimation to 24, 22, and 20 led to a shift in the range of tolerance of the larvae at further stages of development. With a decrease in salinity, acclimated larvae developed more successfully than unacclimated larvae. Acclimated larvae attained the pentactula stage and settled at a salinity range of 32–20; unacclimated larvae, at 32–22. At different stages of development, acclimated larvae survived greater decreases in salinity than unacclimated larvae. The acclimation effects could be traced up to metamorphosis and settling, i.e., two weeks after the end of the acclimation process.     

Chromosome banding in Amphibia

The chromosomes of the South American marsupial frogs Gastrotheca fissipes, G. ovifera, G. walkeri and Flectonotus pygmaeus were analyzed by means of conventional and various banding techniques. The karyotypes of G. ovifera and G. walkeri are characterized by highly differentiated XY/XX sex chromosomes. Whereas the X chromosomes and autosomes contain large amounts of constitutive heterochromatin, extremely little heterochromatin is located in the Y chromosomes. This is in contrast to all previously known amphibian Y chromosomes and the Y chromosomes of most other vertebrates. In the male meiosis of G. walkeri, the euchromatic segments of the heteromorphic XY chromosomes show the same pairing configuration as the autosomal bivalents. The karyotype of F. pygmaeus is remarkable for the unique presence of telocentric chromosomes and the high frequency of interstitially located chiasmata in the meiotic bivalents. The evolution of the karyotypes and sex chromosomes, the structure of the various classes of heterochromatin and the data obtained from meiotic analyses of the marsupial hylids are discussed.     

A model for effective pairing and recombination at meiosis based on early replicating sites (R-bands) along chromosomes

Summary A model for meiotic pairing is proposed in which early replicating sites (R-band equivalent) along chromosomes are envisaged as sites for synaptic initiation. Only within such sites will effective pairing for recombination be established. Pairing in later replicating (G-and C-band equivalent) regions will be ineffective and will not provide for the stringent requirements of the crossover process. Exchange events might be predetermined at S-phase, and possibly at junctions between early and later replicating sequences, these being seen as vulnerable sites for breakage. Temporal shifts in replication from early to late S, are postulated to produce localized pairing disruption and lowering of crossover values as regions of chromatin shift from being effectively to ineffectively paired.     

Premeiosis and meiosis in Lilium “Enchantment”

Various aspects of premeiosis and meiosis in Lilium Enchantment are described. There was evidence of a premeiotic slow-down but no cells in premeiotic despiralization were observed. A relationship was found between sequence of bud development, or reproductive age of the individual, and degree of preleptotene chromosome contraction. The sequence of development of microsporocytes in the anther differed from the apex-to-base order previously reported in Lilium and, in contrast to observations in L. longiflorum cultivars, the maximum degree of preleptotene contraction was found in basal, last developing microsporocytes. Delayed despiralization of telophase nuclei was observed. There were extremely rare cells in meiotic division in anthers in which all other archesporial cells had not yet reached premeiotic interphase. Extreme variation was observed among anthers in proportions of microsporocytes in mid-stages of meiosis as well as in preleptotene contraction. These observations are discussed in relation to meiosis readiness, meiotic behavior in early and late developing regions of reproductive organs and in aging individuals, synchrony of meiotic development and rates of meiotic division.     

Contextualizing Images in Dreams and Daydreams

A contextualizing image (CI) is a powerful central image of a dream which appears to contextualize (provide a picture-context for) the dreamer's emotion. For instance, dreamers who have experienced any serious traumatic event sometimes dream, I was overwhelmed by a tidal wave. This appears to picture their feeling of terror and/or vulnerability.A scoring system for CIs is examined here and is applied to dreams and daydreams supplied by 40 students. Two raters scoring dreams on a blind basis showed good inter-rater reliability. Recent dreams were shown to have more as well as more intense CIs than recent daydreams; likewise, dreams that stand out had more intense CIs than daydreams that stand out. Students with thin boundaries had more and more intense CIs than students with thick boundaries in their recent dreams and nightmare, but not so clearly in dreams and nightmares that stand out. The emotions judged as contextualized by the powerful images tended towards fear/terror and helplessness/vulnerability in dreams (especially in dreams that stand out) whereas emotions contextualized by images in daydreams showed a wide range with no clusters.     

Chromosome banding in Amphibia. XV. Two types of Y chromosomes and heterochromatin hypervariabilty inGastrotheca pseustes (Anura,Hylidae)

The chromosomes of the newly discovered South American marsupial frogGastrotheca pseustes were analyzed by conventional methods and by various banding techniques. This species is characterized by XY/XX sex chromosomes and the existence of two different morphs of Y chromosomes. Whereas in type A males the XY^A chromosomes are still homomorphic, in type B males the Y^B chromosome displays a large heterochromatic region at the long arm telomere which is absent in the X. In male meiosis, the homomorphic XY^A chromosomes exhibit the same pairing configuration as the autosomal bivalents. On the other hand, the heteromorphic XY^B chromosomes form a sex bivalent by pairing their short arm telomeres in a characteristic end-to-end arrangement. Analysis of the karyotypes by C-banding and DNA base pair-specific fluorochromes reveals enormous interindividual size variability of the autosomal heterochromatin.     

Saccharomyces cerevisiae 2-mum DNA. An analysis of the monomer and its multimers by electron microscopy.

Summary The non-tandem inverted duplication in the 2-m DNA of Saccharomyces cerevisiae has a length of 0.19 m and is located asymmetrically along the molecule. The majority of the dumb-bell structures that are formed upon denaturation and selfannealing of the 2-m monomer consists of the renatured inverted duplication sequences as double stranded stem and two single stranded loops of 0.67 m±0.06 m (S-loop) and 0.86 m±0.05 m (L-loop) length. Two additional size classes which comprised 5–10% of the measured molecules had contour lengths of around 1.7 m and 2.1 m. The smaller dumb-bells contained two S-loops and the larger dumb-bells contained two L-loops as was shown by heteroduplex mapping with an HindIII fragment from the L-loop. Two models which assume illegitimate or site specific recombination, are presented to explain the generation of double S-loop and double L-loop molecules. At least part of the 4-m and 6- circular molecules present in the yeast supercoiled DNA fraction are shown to be dimers and trimers of 2-m monomers, but often with inverted loop segments most probably due to intramolecular recombination between sequences of the inverted duplication.2-m DNA is used to indicate the supercoiled DNA fraction although in our measurements the average monomeric length is 1.9 mPart of this work has been presented at the Conference: The Genetics and Biogenesis of Chloroplasts and Mitochondria, Munich, August, 1976