Preferential transposition of aDrosophila P element to the corresponding region of the homologous chromosome

Genetic and physical analyses have demonstrated an intimate interaction or pairing of homologous chromosomes in the nuclei of manyDrosophila cell types. Experiments were performed to determine whether P elements transposing from a given chromosome to its homolog would preferentially insert in the region corresponding to the donor site, perhaps due to such a proximity. AP[lacZ;ry ⁺] element at thecactus locus (35F) on the second chromosome was mobilized and 96 insertions on the homolog were recovered. The distribution of these new insertions was determined by recombination mapping and molecular analysis, and compared with a control set of 93 second-chromosome insertions originating from theX chromosome. A nearly threefold preference was observed for re-insertion in a region of two to three number divisions aroundcactus on the homolog. However, none of these local insertions was actually within 50 kb of the site atcactus corresponding to the starting site. This is in marked contrast to the previously described phenomenon of intrachromosomal local transposition, where the majority of local transpositions are within 10 kb. The data suggest that the mechanisms for intrachromosomal and interchromosomal local transposition are distinct, and are consistent with a model for interchromosomal local transposition involving proximity of homologous chromosomal regions in the nuclei of the germline cells.     

Inference for an age-dependent,multitype branching-process model of mast cells

We consider an age-dependent, multitype model for the growth of mast cells in culture. After a colony of cells is established by an initiator type, the two possible types of cells are resting and proliferative. Using novel inferential procedures, we estimate the generation-time distribution and the offspring distribution of proliferative cells, and the waiting-time distribution of resting cells.List of Notations B _i cumulative distribution function for the time until branching of a cell of type i - b _i probability density function for the time until branching of a cell of type i - b _i b _i (1–D _i ) - D _i cumulative distribution function for the time until death of a cell of type i - d _i probability density function for the time until death of a cell of type i - probability density function of a gamma distribution - G _i cumulative distribution function for the lifetime of a cell of type i - G _1*2 Convolution of G ₁ and G ₂ - ¯G _i 1–G _i - g _i probability density function for the lifetime of a cell of type i - L _i likelihood of a history of type i - m average number of proliferative daughters produced by dividing cells - M _ij (t) the expected number of type-j cells in a colony at time t if that colony began at time 0 with one type-i cell - M _i+ (t) M _i0 (t) + M _i 1(t) + M _i 2(t) - p _rs probability that a dividing cell produces r proliferative and s resting daughters - t _i times defining colony histories. See IV.2.1 - T ₀ time to division of an initiator cell - T ₁, T ₂ times from birth to division of the two daughters of an initiator cell - T ₍₁₎, T ₍₂₎ order statistics of T ₁ and T ₂ - minimum value of a gamma distribution - scale parameter of a gamma distribution or of an exponential distribution - probability per unit time of death for proliferative and resting cells - _rs expected value of p _rs when there is heterogeneity - shape parameter of a gamma distribution     

A statistical model of the reproduction of aphids

1. The logistic function has been generally used to describe the reproductive process of a “population” of animal. However, this model can not give us any information about the reproductive process of “individuals” in the population. In this study a statistical model on the basis of the reproduction of individuals of barley aphid is presented to find the proportion of the mature individuals, the heterogeneity in reproductive ability of the aphids, etc.
2. The model is constructed as follows:
3. The probability that j insects are found on a plant at time t₀ is represented as Q(j).
4. The probability that h individuals of j have reproductive ability, say, mature individuals, in the period t₀ to t₁ is represented as B(h/j)=_jC_hw^h(1−w)^j−h, where w is the proportion of mature individuals.
5. In a population with a homogeneous reproductive ability, the probability that each parent lays i offspring in the period t₀ to t₁ is represented as P(i/m)=e^−mmⁱ/i!, where m is mean. And, in a population, m changes according to the gamma distribution. Hence the probability that a parent lays i offspring between t₀ and t₁ is represented as , where p and k are parameters of negative binomial distribution. The probability that h parents on a plant lays s offspring is represented as .
6. From the assumptions mentioned above, the probability that s offspring are to be found at time t₁ on a plant with the original j individuals at time t₀ is represented by
7. The experimental populations were demonstrated to fit well to the model.

     

Transposition of mobile elements gypsy (mdg4) and hobo in germ-line and somatic cells of a genetically unstable mutator strain of Drosophila melanogaster.

Summary Using the in situ hybridization technique, we have analysed the distribution of mobile elements in the X chromosomes of male offspring of individual mutator strain (MS) males crossed to attached-X females. The experiments demonstrate varying cytological localization of the mobile elements gypsy (mdg4) and hobo among different individuals. The other mobile elements investigated (mdgl, mdg3, 412, 297, copia, 17.6, Doc, H.M.S. Beagle, Springer, FB) display no changes in insertion sites. Such an experiment is equivalent to analysis of separate gametes of an MS individual. Thus, the ability of gypsy and hobo to transpose in germ-line cells is demonstrated directly. Transpositions occur at premeiotic stages of germ cell development, since they appear in clusters. Analysis of gypsy and hobo transposition events shows that they occur independently. The same experiment demonstrates that gypsy localization varies significantly between different salivary gland cells of an MS individual. Two types of gypsy hybridization sites can be distinguished: permanent sites, common to all cells, and additional ones varying between neighbouring salivary gland cells. These additional sites indicate gypsy transposition in somatic cells of the MS. Transposition of the hobo element in somatic cells has also been observed.     

A model of the plant-to-plant movement of aphids I. Description of the model

The plant-to-plant movement of insects in one of the factors determining the distribution of individuals in insect populations. In this report the movement of barley aphids was analyzed by a statistical model. The model is represented as the convolution of three probability functions:

1. The probability that s individuals are found on a plant at time t₀:Q(s);
2. The probability that i individuals leave the plant and remain on the ground from time t₀ to t₁:_sC_ipⁱq^s−i and p+q=1, where p and q are the proportions of individuals which do not leave a plant and which leave it once or more, respectively;
3. The probability that j individuals climb a plant between time t₀ to t₁ and stay there at time t₁:e^−λλ^j/λ^!, where λ is the mean of the individuals.

The probability that l individuals are located on a plant at time t₁ is represented by the following equation It was shown by simple experiments that the experimental populations were well fitted to the model.     

Transposon Tn1 intra-molecular transposition

Summary A system for the direct selection of intra- and inter-molecular transposition events has been used to show that intra-molecular transposition of Tn1 generates deletions and inversions and requires the tnpA but not the tnpR gene product, as predicted by current models of transposition. Intra-molecular Tn1 transposition is much less limited by transposition immunity than inter-molecular transposition, and occurs at frequencies comparable to those for inter-molecular transposition. The selection system, which uses the bacteriophage cI-P_R region as a target can be used to select, quantify, and characterize any spontaneous or induced mutations.     

“Cryptic” dinucleotide polymorphism in the 3′ region of the factor IX gene shows substantial variation among different populations

Long tandem dinucleotide repeats composed of alternating purines and pyrimidines [RY(i)] are abundant and highly polymorphic. Simple RY(i) are predominately composed of one tandem repeat of a dinucleotide sequence. In contrast, cryptic RY(i [cRY(i)] are composed of multiple short dinucleotide repeats. Herein, we describe the racial distribution of alleles for a polymorphic cRY(i) in the factor IX gene. Allele I is absent in Asians, whereas allele III is rare or absent in Caucasians or blacks. A polymorphic cRY(i) analyzed previously shows even more dramatic variation among racial groups, hinting that a battery of cRY(i) might have utility in assessing the racial origin of a DNA sample.     

Genetic evaluation with autosomal and X-chromosomal inheritance

Summary At present, genetic evaluation in livestock using best linear unbiased prediction (BLUP) assumes autosomal inheritance. There is evidence, however, of X-chromosomal inheritance for some traits of economic importance. BLUP can accommodate models that include X-chromosomal in addition to autosomal inheritance. To obtain BLUP with autosomal and X-chromosomal additive inheritance for a population in which allelic frequency is equal in the sexes, and that is in gametic equilibrium, we write y _i = x_i + a_i + s_i + e_i, where y _i is the phenotypic value for individual i, x_i, is a vector of constants relating y _i to fixed effects, is a vector of fixed effects, a _i is the additive genetic effect for autosomal loci, S _i is the additive genetic effect for X-chromosomal loci, and e _i is random error. The covariance matrix of a _i's is A _A ² , where A is the matrix of twice the co-ancestries between relatives for autosomal loci, and _A ² is the variance of additive genetic effects for autosomal loci. The covariance matrix of s _i's is S _F ² , where S is a matrix of functions of co-ancestries between relatives for X-chromosomal loci and _F ² is the variance of additive genetic effects for X-chromosomal loci for noninbred females. Given the covariance matrices of random effects a _i, s_i, and e _i, BLUPs of autosomal and of X-chromosomal additive effects can be obtained using mixed model equations. Recursive rules to construct S and an efficient algorithm to compute its inverse are given.Dedicated to the memory of Dr. C. R. Henderson, whose encouraging comments stimulated the research in this paper. Supported in part by the Illinois Agricultural Experiment Station, Hatch Project 35-0367, Estimation of Genetic Parameters.     

Induction of MGE 412 Transposition in an Isogenic Strain of Drosophila melanogaster by Different Doses of Ethanol Fumes

The effect of treatment of males from an isogenic Drosophila melanogaster strain by limiting doses of ethanol fumes on transpositions of MGE412 was examined. Validity of the phenomenon of transposition induction was demonstrated. We estimated rates of induced transposition (10^–2 events per site, per sperm, per generation versus <10^–3 in control) and showed dose dependence of the rate on the exposure time of the males to ethanol fumes. Experiments with alcohol treatment at limiting doses must end either in death of the individuals or bursts of genetic variability in their progeny. In terms of genetics of an individual, this may mean loss of vital hereditary basis followed by mass degradation of the progeny of the hard drinkers. In terms of populations genetics, this mode of MGE transposition induction can rapidly create a burst of novel genetic variation, which, apart of great losses, may generate a number of advantageous individuals, i.e., be significant for population survival in new, stressful environments.     

An interchromosomal gene conversion of the Drosophila dunce locus identified with restriction site polymorphisms: a potential involvement of transposable elements in gene conversion

Summary Females heterozygous for the two alleles dnc ² and dnc ^M14 of the X-linked gene dunce (dnc), and carrying a copy of dnc ⁺ progeny X-chromosomes from recombination experiments. Restriction site polymorphisms have been used as genetic markers to follow the parentage of dnc locus segments in these chromosomes. All six chromosomes are identical with respect to the spectrum of restriction site markers they carry in the dnc ⁺ chromosomal region. In the progeny chromosomes, this region is comprised of sequences like the dnc ^M14 X-chromosome and the translocation copy of dnc ⁺. Sequences flanking the dnc gene in the progeny chromosomes are like the dnc ^M14 chromosome. Internal to the gene but near the 5 end, is a segment from the dnc ⁺ translocation which has apparently originated from an interchromosomal and premeiotic gene conversion event. In addition, two transposable elements have inserted into the progeny chromosomes, one towards the 5 end of dnc and the other near the 3 end. The insertion of these elements occurred premeiotically since all six chromosomes are structurally identical. The data are interpreted with respect to a potential role of transposable element transposition in the process of gene conversion.     

Detection of chemicals that stimulate Tn9 transposition in Escherichia coli K12

Summary A spot test has been developed for detecting substances that enhance the transposition of Tn9 in Escherichia coli. Phage :: Tn9-infected cells were plated on chloramphenicol media and a drop of the test substance was placed at the center of the plate. Following incubation, chloramphenicol-resistant colonies appeared due to the transposition of Tn9 to the bacterial chromosome. By comparing the test plate and a control plate with respect to the number and distribution of colonies, the effect of the test compound can be evaluated.Out of over 100 compounds tested, acetate, two detergents (Brij 58 and Nonidet P40) and dimethylsulfoxide were found to enhance transposition 3–20 fold. Acetate was also found to enhance the transposition of Tn5 and Tn10. The stimulating effect of Brij 58 was lost when palmitic acid was added with the Brij 58. The nature of these substances, which we refer to as transposagens, suggests an involvement of lipid or membrane in the transposition process.Abbreviations AMP-R, CAM-R, KAN-R, SPC-R, TET-R resistance to ampicillin, chloramphenicol, kanamycin, spectinomycin and tetracycline, respectively - DMSO dimethylsulfoxide A preliminary report of this work was presented at the Fifth Mid-Atlantic Extrachromosomal Genetic Elements Meeting, 1981 (Datta, Randolph and Rosner, Plasmid 7:99, 1982)     

Tolerance regions with segmented fermentation processes

Many microbial fermentation processes exhibit different phases (e.g. adaption phase, main growth phase, main production phase). The process variables e.g. the biomass vary randomly about their mean. The experimentalist is interested to know the break points of the different phases, and a tolerance region, i.e. a range of possible values of the process variable that can be considered as normal. This paper deals with statistical methods for determining break points and tolerance regions.List of Symbols a _i intercept in phasei - b _i specific growth rate in phasei - e _t deviation of a measurement in timet - tEX expectation of variableX - r number of phases of fermentation - T _i break point of phaseit - t _ij time of measurementj in phasei - t _n–2.1–/2 quantile oft distribution - Y(t) logarithm of measurement at timet Greek Letters 1 – cover probability of tolerance region - 1 – part covered by the tolerance region - ² variance ofe _t - (·) standard normal distribution - quantile of chisquare distribution     

Optimal and central-place foraging theory applied to a desert harvester ant,Pogonomyrmex californicus

Summary Certain predictions of optimal- and central place-foraging theory were tested on the desert harvester ant, Pogonomyrmex californicus. Colonies were offered three different sizes of oat seed and found to maximize net energy intake (ei) over time (t _i ) by harvesting the seed sizes with the highest e _i /t _i rank. Two aspects of t _i were measured that were assumed constant in previous studies. The handling components of t _i (time required to manipulate the seed and travel time back to the colony with the food) were measured and found to be positively correlated with seed size. The manipulation success rate (the percentage of handled seeds successfully picked up) decreased with increased seed size. These results point out how important it is to measure all parameters of e _i /t _i rather than to assume constancy with both prey type and foraging distance. The relative abundance of less preferred food types was important in determining the proportion of preferred types in the diet. The food supply of eight colonies was manipulated experimentally over a 25-day period. Four deprived colonies were constrained within aluminum enclosures to prevented foraging. The remaining four satiated colonies were given food ad libitum. The niche breadths of the treated colonies were then compared to controls, but found not to differ significantly. Seed baits were offered at three distances from the colony to test whether selectivity increased with disance. Contrary to theoretical predictions, all colonies harcested about the same proportion of each seed size at each distance.     

Transposition pattern of a modified Ds element in tomato

Several aspects of transposition of an in vitro modified Ds element are described. This Ds element, designated ds-r, is equipped with bacterial plasmid sequences and can, therefore, be rescued from the plant genome. Our results indicate that the Ds-r element has a late timing of transposition from T-DNAs. This feature of the element might be advantageous for tagging experiments because it leads to independently transposed germinally transmitted elements. Furthermore, it is shown that Ds-r transposition generates clusters of insertions, indicating that genes to be tagged should be located in genomic regions covered by insertions.     

Biochemical analysis of isoallelic series at the al- i locus of Neurospora crassa

The neutral carotenoids of 3 phenotypically distinct albino-1 (al- i) strains, a wild type, 2 heterokaryons containing 2 al- i, alleles and 1 heterokaryon containing al- i+al-2 markers were analyzed. All al- i strains and the al- i heterokaryons contained large amounts of phytoene and only traces of higher carotenoids such as -carotene and lycopene which are responsible for the phenotypic variation at this locus (from pure white to lemon yellow). The biochemical lesion for al- i mutants affects phytoene dehydrogenase and enzyme leakiness accounts for the gene polymorphism. There is no evidence for interallelic complementation at the al- i locus.     

Analyses of<Emphasis Type="Italic"> cis</Emphasis> -acting elements that affect the transposition of<Emphasis Type="Italic"> Mos1 mariner</Emphasis> transposons in vivo

The left (5) inverted terminal repeat (ITR) of the Mos1 mariner transposable element was altered by site-directed mutagenesis so that it exactly matched the nucleotide sequence of the right (3) ITR. The effects on the transposition frequency resulting from the use of two 3 ITRs, as well as those caused by the deletion of internal portions of the Mos1 element, were evaluated using plasmid-based transposition assays in Escherichia coli and Aedes aegypti. Donor constructs that utilized two 3 ITRs transposed with greater frequency in E. coli than did donor constructs with the wild-type ITR configuration. The lack of all but 10 bp of the internal sequence of Mos1 did not significantly affect the transposition frequency of a wild-type ITR donor. However, the lack of these internal sequences in a donor construct that utilized two 3 ITRs resulted in a further increase in transposition frequency. Conversely, the use of a donor construct with two 3 ITRs did not result in a significant increase in transposition in Ae. aegypti. Furthermore, deletion of a large portion of the internal Mos1 sequence resulted in the loss of transposition activity in the mosquito. The results of this study indicate the possible presence of a negative regulator of transposition located within the internal sequence, and suggest that the putative negative regulatory element may act to inhibit binding of the transposase to the left ITR. The results also indicate that host factors which are absent in E. coli, influence Mos1 transposition in Ae. aegypti.Communicated by G. P. Georgiev     

On coenzyme Q orientation in membranes: A linear dichroism study of ubiquinones in a model bilayer

Summary A general approach is developed to interpret linear dichroism (LD) spectra of ubiquinones (Q _n) in host bilayers. Information is reported in terms of guest-host mutual orientation and localization. The overall orientational anisotropy of guest ubiquinone molecules is described by a basic set of limiting orientation/localization modes. Assignments of the UV transitions of the ubiquinone chromophore were obtained by the liquid crystal-linear dichroism technique and molecular orbital (CNDO/S) calculations. The LD spectra of Q _n in the bilayers provided by the lyotropic nematic mesophase exhibited by water solutions of potassium laurate and decanol were interpreted on the basis of the above assignments. The resulting experimental evidence showed a multisite distribution in the host bilayer for the aromatic heads of all the investigated Q _n derivatives except Q₀. The orientational distribution suggested by the LD spectra fits the solubilization model recently proposed by G. Lenaz [J. Membrane Biol. (1988) 104:193–209] for ubiquinone in lipid membranes. Within this model Q _n molecules are located in the midplane and their headgroups oscillate transversally across the membrane. Q ₀ instead has a single site location, close to the polar bilayer interface. Experimental evidence that the headgroup carbonyls tend to grasp the polar interface of the host bilayer was also obtained. Orientation and location distributions of Q _n guest molecules are therefore likely to result from the tendency of their aromatic heads to grasp the polar heads of the host bilayer and from the concurrent tendency of their chains to settle into the hydrocarbon host interior.abbreviations AA average absorption - OD, OD optical densities for plane polarized radiations parallel () and perpendicular () to the sample optical axis - OD OD — OD - EPR electron paramagnetic resonance - LC-LD liquid crystal-linear dichroism - LD linear dichroism - LD _r reduced linear dichroism. - MO molecular orbital - N nematic - NMR nuclear magnetic resonance - S _jj order parameters of the directions j of the transition moments of the guest chromophore - S _ii order parameters of the orientational axes i of the guest molecule with respect to the magnetic field - S _ii order parameters of the axes i of the guest molecules with respect to the bilayer axis a - S _a order parameters of the host bilayer axis a with respect to the orienting magnetic field - _j,i deflection angles between the directions j and the axes i - O _i optical factors of the i axis see Eq. (A4)] - Q_n ubiquinone whose isoprenoid chain contains n isoprenoid units Dr. A. Rossi is gratefully acknowledged for the t.e.m. reduction of the spectra. Ubiquinone homologs were kind gifts from Eisai Co., Tokyo, Japan. This work was supported by M.U.R.S.T., and C.N.R. Target Project on Biotechnology and Bioinstrumentation, Rome, Italy.     

Prolongation of MGE 412 Transposition Induction after γ-Irradiation in an Isogenic Line of Drosophila melanogaster

The dose dependence of the rate of -induced transpositions and consequent dynamics of the MGE 412pattern after -irradiation were investigated in isogenic line 49 in generations F₁, F₁₂, F₁₄₀, and F₁₇₀. It was shown that the results on dose dependence of transpositions was very similar with the corresponding results of the classic works by Timofeeff-Ressovsky et al.(1935). It is suggested that the transcribed copies of retrotransposon 412cure -radiation-induced double-strand DNA breaks. The phenomenon of prolongation of MGE transposition induction during early generations after treatment was shown. In this period (F₁–F₁₂), the maximum transposition rate ( 2 × 10^–2events per MGE copy, per haploid genome, per generation) and the maximum number of heterozygous MGE copies were achieved. In the late generations (F₁₄₀–F₁₇₀), the reduced induction level ( 10^–3) was established. In the population of effective size N _e= 2000 individuals, this corresponds to the state when 1/4N _e, i.e., when the transposition flow prevails over the MGE copy loss by genetic drift. These data together with some indirect evidence argue for the hypothesis that the spontaneous transposition rate is proportional to the average number of heterozygous MGE copies per diploid genome.     

Regression analysis of yield stability is strongly affected by companion test varieties and locations — examples from a study of Nordic barley lines

The suitability of regression analysis for studying the phenotypic stability of grain yield was investigated using a collection of 220 Nordic barley lines. Linear regression explained 26–52% of the genotype x environment (GE) interactions in different groupings of the material. The regression coefficient, b _i , measures the yield response of the i-th genotype to improved environmental conditions. Deviations from regression, S _di ² , have been used to estimate Tai's stability parameter, _i , which is a measure of the phenotypic yield stability in the agronomic sense. Repeatability of b _i , _i , and grain yield was studied by means of correlations between estimates obtained in each experimental year. Yield had the highest repeatability, with correlations between years ranging from 0.57 to 0.85. In this study, regression coefficients and _i -values were not repeatable, i.e. genotypes reacted differentially to the yearly climatic variations. Six-rowed (6r) barleys had higher responsiveness, but lower mean yields, than two-rowed (2r) barleys. This is partly due to the history of selection of 6r-barleys, which mainly originate from regions with low potential yield levels, i.e. Finland and Norway. In general, responsiveness and stability were not correlated with yield. The highest-yielding lines had b _i 1. The response pattern of the different types of barleys used in this study show that responsiveness can be changed by recombination.