Developmental profiles of three embryo-lethal maize mutants lacking leaf primordia: ptd*-1130, cp*-1418, and bno*-747B

The defective kernel (dek) mutants of maize are altered in both their embryo and endosperm development. Earlier studies have indicated that some of the dek mutants are unable to form shoot apical meristems or leaf primoirda. We have examined three embryo lethal dek mutants of this type, ptd*-1130, cp*-1418, and bno*-747B, to obtain a developmental profile for each. Allelism tests show that these three mutants are not allelic. Embryos were examined in early, mid-, and late kernel development as well as at kernel maturity by dissection and sectioning procedures and also at kernel maturity by scanning electron microscopy. All three mutants lag behind normal embryos in their rate of development. Embryos of ptd*-1130 reached the transition stage by early kernel development and progressed no further but underwent cell enlargement and necrosis during late kernel development. Embryos of cp*-1418 reached an early coleoptilar stage by midkernel development. They subsequently increased in size but did not form any leaf primordia. At kernel maturity, they no longer had a shoot apical meristem but often had a well formed root meristem. They appeared to remain healthy and did not become necrotic. Embryos of bno*747B reached the early coleoptilar stage by early kernel development but progressed no further. By kernel maturity, they had grown into masses of irregularly shaped embryonic tissue that no longer resembled any normal embryo stage but were not necrotic. None of these three mutants responded to attempts to support continued embryo development when cultured, but all three mutants formed callus on N6 and MS media supplemented with 2,4-D. These results indicate that these mutants are all uniformly blocked at specific stages early in embryonic development, have different subsequent developmental fates, and represent three different genes performing unique functions that are essential for embryogenesis.     

The expression of human glycerol-3-phosphate dehydrogenase in human/rodent somatic-cell hybrids

Our previous studies using rodent/human somatic-cell hybrids suggested that the expression of human mitochondrial glycerol-3-phosphate dehydrogenase (GPDM) is dependent on the presence of human mitochondria. This has now been tested directly by analysis of GPDM activity in a series of nine hybrid-cell lines, four segregating human chromosomes and five losing rodent chromosomes (reverse segregants). The chromosome composition of the hybrids was deduced from analysis of biochemical markers and examination of G- and G11-banded metaphase spreads and the mitochondrial content was determined by Southern blot analysis, using cloned mouse and human mtDNA sequences as probes. We found that the mtDNA species present in these hybrids correlated exactly with the pattern of chromosome segregation such that the conventional hybrids contained rodent mtDNA and the reverse segregants human mtDNA. However, the pattern of GPDM expression was not directly correlated with the species of chromosomes or mitochondria present: all the hybrids showed strong rodem GPDM activity and two from each class of hybrid also showed human GPDM activity but the other hybrids were negative for human GPDM. We conclude that rodent GPDM readily integrates into human mitochondria, that the expression of rodent GPDM is not dependent on the presence of rodent mitochondria, and that GPDM is not coded by mtDNA. Human GPDM either is not capable of being inserted into the rodent mitochondrial membrane or is regulated in some way in the hybrid cells by an unidentified rodent factor.     

Locus determining the human sperm-specific lactate dehydrogenase,LDHC, is syntenic with LDHC

From the data presented in this report, the human LDHC gene locus is assigned to chromosome 11. Three genes determine lactate dehydrogenase (LDH) in man. LDHA and LDHB are expressed in most somatic tissues, while expression of LDHC is confined to the germinal epithelium of the testes. A human LDHC cDNA clone was used as a probe to analyze genomic DNA from rodent/human somatic cell hybrids. The pattern of bands with LDHC hybridization is easily distinguished from the pattern detected by LDHA hybridization, and the LDHC probe is specific for testis mRNA. The structural gene LDHA has been previously assigned to human chromosome 11, while LDHB maps to chromosome 12. Studies of pigeon LDH have shown tight linkage between LDHB and LDHC leading to the expectation that these genes would be syntenic in man. However, the data presented in this paper show conclusively that LDHC is syntenic with LDHA on human chromosome 11. The terminology for LDH genes LDHA, LDHB, and LDHC is equivalent to Ldhl, Ldh2, and Ldh3, respectively.     

NMR, CD and IR spectroscopies of a tridecanucleotide containing a no-base residue: coexistence of B and Z conformations.

The synthesis of the tridecadeoxynucleotide d(CGm5CGCGxACATGT), where x is the 1-cyano-2-deoxy-beta-D-erythropentofuranose, is described. The NMR, IR, CD studies at various salt concentrations and temperatures of this oligomer show that the B and Z conformations are simultaneously present in the same short DNA fragment. A single apurinic residue is sufficient for the coexistence of the B and Z helices on this oligomer.     

Eine nicht-reziproke Kreuzungssterilität zwischen ökologischen Rassen der Mücke Clunio marinus

Zusammenfassung Die in der Gezeitenzone lebende Mücke Clunio marinus ist längs der europäischen Küstenlinie verbreitet. Die experimentell geprüften Stämme verschiedener geographischer Herkunft repräsentieren ökologische Rassen, die sich in der zeitlichen Programmierung ihrer Entwicklung unterscheiden. Es wurde die Kreuzbarkeit zwischen insgesamt 7 Stämmen geprüft.Zwischen einzelnen Stämmen wurde eine nicht-reziproke Kreuzungssterilität (abgekürzt n.r.St.) nachgewiesen, bei der jeweils in einer Kreuzungsrichtung fertile Nachkommen entstanden und in der reziproken Kreuzung Nachkommen fehlten.Die Vererbung der n.r.St. wurde zwischen 2 Stämmen benachbarter Rassen mit der Methode der wiederholten Rückkreuzung geprüft. Es ergab sich ein matrokliner Erbgang. Die Befunde werden mit entsprechenden Ergebnissen von Laven an Culex pipiens verglichen.Die populationsgenetischen Konsequenzen der n.r.St. werden in Hinblick auf die Elimination von Kreuzungstypen, Genfluß und reproduktive Isolation betrachtet. Für die Bedeutung der n.r.St. im Freiland werden 3 Hypothesen erörtert: 1. Begleiterscheinung der genetisch divergierenden Rassen, 2. in einer Richtung wirksamer Isolationsmechanismus zwischen benachbarten Rassen und 3. Speciation.

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Summary The intertidal midge Clunio marinus is distributed along the European coast-line. Stocks from distinct locations differ in the programming of their emergence time. They represent ecological races. The crossability between 7 stocks was examined.Between some stocks a non-reciprocal cross sterility has been found, characterized by fertile hybrids in one cross direction, and no offspring in the reciprocal crosses.The cross Jean xSan was fertile, while the cross San xJean was sterile. After three backcrosses of the hybrid females to San males, the sterility in the reciprocal crosses with San females had not been changed. The maternal inheritance of this non-reciprocal sterility is compared with similar studies in Culex pipiens by Laven.According to aspects of population genetics, the non-reciprocal cross sterility is considered in view of elimination of crossing types, of gene flow and reproductive isolation. With regard to the significance of the non-reciprocal cross sterility in the field, three hypotheses are discussed: 1. by-product of evolutionary divergence in ecological races, 2. unilateral reproductive isolation which blocks the gene flow between adjacent populations only in one direction, and 3. speciation.

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Mit Unterstützung durch die Deutsche Forschungsgemeinschaft.

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Herrn Professor Dr. Gerhard Krause zu seinem 65. Geburtstag.     

Metastable secondary structures in ribosomal RNA: a new method for analyzing the titration behavior of rRNA

The pH titration behavior of E. coli rRNA in the acid range has been analyzed by combining spectrophotometric and potentiometric titration data. The “simplest” model for the system, which considers as possible reactions the protonation of adenine (A), cytosine (C), and guanine (G) residues along with the opening of A·U and G·C base pairs, does not adequately account for the titration properties. It is postulated that extra reactions may occur in addition to those in the “simplest” model, and a new analytical method was developed to deal with this situation. Our approach yields the ultraviolet spectral changes which accompany the extra reactions, from which the nature of these reactions can in principle be deduced. The calculations also give, at each pH, the extents of the extra reactions as well as the extents of those reactions which comprise the “simplest” model. We infer that in acidic RNA solutions of 0.1M ionic strength there occur at least two extra reactions, each of which involves G residues. We propose that in the pH range 6.0 ≥ pH ≥ 3.8 triple-stranded helical sequences, presumably protonated G·C·G, are formed. These regions are replaced at lower pH by acid-stable structures involving G·G and A·A base pairs. In solutions of lower ionic strength (I = 0.01M) no triple strands are formed, but G·G and A·A regions seem to develop even at pH values as high as 6.0. At I = 0.1M, an acid–base titration cycle between pH 7 and 2.8 is not reversible; rRNA shows true hysteresis behavior. We conclude that in ribosomal RNA's, which are generally G-rich, guanine residues may participate in hitherto unpredicted conformations, some of which may be metastable while others are equilibrium structures.