Unusual occurrence of aldehydes and ketones in the defensive secretion of the tenebrionid beetle, Eleodes beameri

The defensive secretion of the tenebrionid beetle, Eleodes beameri, is quite unlike the benzoquinone and 1-alkene secretion of other species of Eleodes and Tenebrionidae. Twenty-three compounds were isolated from the secretion by gas-liquid chromatography (GLC) and 13 of these were identified by infrared, nuclear magnetic resonance, ultraviolet, and mass spectroscopy. Identified compounds were: 1-nonene (3·2%), 1-undecene (<0·5%), n-hexanal (15·6%), n-heptanal (0·9%), n-octanal (4·5%), trans-2-hexenal (2·0%), trans-2-heptenal (1·5%), trans-2-nonenal (28·6%), trans-2-decenal (3·4%), n-3-nonanone (0·5%), n-1-nonen-3-one (16·8%), methyl-1,4-benzoquinone (22·0%), and 1-hexanol (<0·5%). 1-Nonen-3-one is unique to E. beameri. A number of minor components remain unidentified. The morphology and ultrastructure of the glands were similar to other species of Eleodes. The gland reservoirs are a pair of strongly bilobed sacs with narrow exit ducts opening between abdominal sternites 7 and 8. There are two types of secretory cell units: Type 1 consisting of cells closely attached to the reservoir intima, with large, central vesicles drained by highly convoluted tubules. Type 2 units are composed of a pair of cells functioning together, the cuticular organelle from the microvilli-filled vesicle of the distal cell (2a) passing through the vesicle of the proximal one (2b) and then draining more or less directly into the reservoir via a cuticular tubule.     

Further evidence and biological significance for non-random localization of the centromere on mammalian chromosomes

A further quantitative analysis of the localization of the centromere on chromosomes was made using 16,817 individual chromosomes obtained from 723 mammalian species. Centromeric position was expressed quantitatively by the size of short arms as per cent weight (S_w) relative to the X-containing haploid set. When the class interval of S_w was 0·1 instead of the previous 0·2 (Imai, 1975), the frequency distribution of S_w showed an uneven (W-shaped) pattern with two distinct antimodes lying at S_w 0·6 (reconfirmation) and 0·1 (new finding). Two hypotheses, that are not mutually exclusive, are proposed to explain the non-random distribution of centromere position. One is that there are three structurally different short arms consisting of (1) centromere, (2) constitutive heterochromatin (as determined by C-banding), and (3) euchromatin, each arm-type being approximately characterized by the size of short arms (S_w) as S_w < 0·1, 0·1 ? S_w ? 0·6 and S_w > 0·6. The other possibility is concerned with an “orthogenetical” change of chromosome morphologies. When the chromosomes with S_w < 0·1, 0·1 ? S_w ? 0·6 and S_w > 0·6 are denoted as telocentric (T), acrocentric (A), and meta-, submeta- and subtelocentric (M, SM & ST), it was suggested that the chromosome morphologies tend to change orthogenetically (in a statistical sense) from T to M, SM & ST via A-chromosomes by rearrangements such as tandem growth of constitutive heterochromatic, pericentric inversions, and centric fusions.     

Effects of fermenter type,xylanase addition and dual cultures on fungal fermentations of wheat pollard and bran

Pollard and bran were fermented by a selection of filamentous fungi to increase the protein content and availability for use as animal feed. Aspergillus terreus produced a product containing 32·6% crude protein (CP) after 16 days. Under identical environmental conditions, shallow-layer solid-state fermentations achieved higher CP yields than did tumbled or packed-column systems. When crude xylanase was added with A. terreus inoculum, a 5-day reduction in fermentation time was achieved resulting in a maximum CP content of 27%. A. terreus, Chaetomium virescens, Schizophyllum commune or Trichoderma reesei, in dual culture with one another or in combination with Phanerochaete chrysosporium, did not achieve higher final CP yields (after 16 days) than A. terreus alone. P. chrysosporium in combination with T. reesei and with S. commune resulted in the most rapid CP development of 26·1% and 26·4%, respectively, during the first 10 days.     

Non‐Tuberculosis mycobacterium speciation using HPLC under Revised National TB Control Programme (RNTCP) in India

Aims

Non‐Tuberculous Mycobacteria (NTM) are ubiquitous in nature. The data on prevalence of NTM under the RNTCP is scarce. Many NTM species have clinical significance, and hence their identification and speciation are important.

Methods and Results

It is a cross‐sectional study conducted at the five RNTCP accredited culture and drug susceptibility testing (CDST) laboratory. The culture isolates from AFB positive but Immunochromatographic test negative samples were taken for identification and speciation using HPLC. Of the total 266 isolates only 164 isolates had a second sample received at the laboratory. The speciation was done using HPLC for those isolates. The type of species identified are: 26·8% (44) were Mycobacterium chelonae, 12·8% (21) were Mycobacterium fortuitum, 9% (15) were Mycobacterium gordonae, 9% (15) were Mycobacterium tuberculosis complex, 6·1% (10) were Mycobacterium kansasii, 4·9% (8) were Mycobacterium simiae, 2·4% (4) were Mycobacterium thermophile, 1·2% (2) were Mycobacterium gastri, 0·6% (1) were Mycobacterium scrofulaceum, 0·6% (1) were Mycobacterium avium and 4·9% (8) isolates had chromatogram which was un‐interpretable.

Conclusion

Identification and its speciation of NTM are not routinely done under TB control programme. Since HPLC could identify 95% of isolates belonging to 10 species, the speciation of NTM using HPLC should gain importance in the diagnosis of disease caused by NTM.

Significance and Impact of Study

NTM are emerging as important causative agents of pulmonary and extra pulmonary disease, the ability to recognize disease caused by NTM and subsequently treat such disease has become increasingly important. The identification of NTM up to its species level should gain importance in all TB reference Laboratories.     

Clearance rates of sessile rotifers: In situ determinations

Clearance rates of three sessile and four free-swimming rotifer species from a small acid bog-pond were measured using in situ techniques. Three radioactively labeled cell types, an alga (Chlamydomonas), a bacterium (Enterobacter = Aerobacter), and a yeast (Rhodotorula) were used as tracers. Clearance rates (using yeast) ranged from <1.0 to >250 µl · animal^?1 · h^?1 depending on species. Ptygura crystallina, Ptygura pilula, Floscularia conifera, and an unidentified bdelloid ingested all three foods with substantial variation in clearance rates among species and cell type. There was an insignificant error (<0.3%) in clearance rate associated with non-ingestive uptake of radioactivity. Among the free-swimming taxa, Lecane sp. had a clearance rate of <0.5 µl · animal^?1 · h^?1 on yeast, while another Lecane sp. and Trichotria tetractis did not ingest that cell type.     

Gas exchange characteristics of Gulf of Mexico coastal marsh macrophytes

Gas exchange characteristics of three major Louisiana Mississippi River deltaic plain marsh species, Spartina patens (Ait.) Muhl., Spartina altemiflora Lois., and Panicum hemitomon Shult., was studied under controlled environment conditions. The optimum temperature for maximum photosynthesis was ≈ 36 °C for S. patens, 27 °C for S. alterniflora, and 28 °C for rP. hemitomon. Net photosynthesis rates at optimum temperature averaged 20.1 μmol · m^t-2 · s^t-1 in S. patens, 22.8 μmol · m⁻² · s⁻¹ in S. alterniflora, and 11.4 μmol · m⁻² · s⁻¹ in P. hemitomon. Photosynthetic light saturation occurred ≈720, 530, and 750 μmol · m⁻² · s⁻¹ in S. patens, S. alterniflora, and P. hemitomon, respectively. Only S. patens had a midday depression of stomatal conductance, but net photosynthesis was not reduced by the depression. Maximum stomatal conductances were 285 mmol · m⁻² · s⁻¹ in S. patens, 238 mmol · m⁻² · s⁻¹ in S. alterniflora, and 335 mmol · m⁻² · s⁻¹ in P. hemitomon. In contract, net photosynthesis values were lower in P. hemitomon compared with the Spartina species, indicating a greater degree of water use efficiency of photosynthesis for both Spartina species.     

Efficiency of biomass transfer and the stability of model food-webs

Low efficiency of biomass transfer between trophic levels was found to enhance the stability of a model ecosystem in Lotka-Volterra form, consisting of six basal species, three primary consumers and an omnivore (De Angelis, 1975). The present paper extends De Angelis's result to a more general class of models, varying in species number, connectance and precise features of web design. Whilst the efficiency of biomass transfer does influence stability, it does not do so in the relatively simple way proposed by De Angelis. Three ranges of maximum efficiency of biomass transfer, γ_max, were employed, biologically probable (1 > γ_max > 0· 1), possible to very unlikely (0 · 1 > γ_max>0 · 01) and highly improbable (0.01> γ_max> 0· 001). Over most web configurations, in biologically probable regions of ymax, increasing connectance decreased the probability of webstability—the opposite of De Angelis's prediction. Increasing connectance only enhanced stability in biologically unrealistic regions of γ_max. Stability was also markedly influenced in these models by the number of component species and trophic levels in the web, features not evaluated by De Angelis. Low efficiency of biomass transfer enhanced stability in some types of web, but not in others.     

Isolation and characterization of dinoflagellate and chrysophyte cytochrome-f (553–4)

Cytochrome-f (553–4) was isolated from mass cultures of the six dinoflagellates, Amphidinium carterae (2 strains), Cachonina niei, Glenodinium sp., Peridinium foliaceum, Gonyaulax polyedra, and one chrysophyte, Cricospherae carterae. Sonication of whole cell suspensions released the water-soluble protein, which was then purified by vacuum dialysis, salt fractionation and column chromatography. Reduced forms of isolated cytochromes had absorption maxima at 270–6, 316–8, 415–6, 522–3 and 553–4 rim. The α-absorption peak was asymmetrical. MW's, as determined by SDS polyacrylamide gel electrophoresis, ranged from 10 700 to 13 500. Amino acid analysis of C. niei cytochrome-f revealed 102 residues, with a composite MW of 10836. Purified cytochromes had isoelectric points ranging from 3·45 to 4·25 and oxidation-reduction potentials ranging from +0·374 to +0·351 V.     

The susceptibility of Apodemus agrarius and Rattus losea to the anticoagulant rodenticide,flocoumafen

Flocoumafen had good rodenticidal action against Apodemus agrarius and Rattus losea. The acute oral LD₅₀ for male A. agrarius and R. losea was 1·22 mg kg⁻¹ and 1·36 mg kg⁻¹ respectively. Flocoumafen bait was more toxic to R. losea than to A. agrarius. At bait concentrations of 0·002–0·005%, flocoumafen had a single-feed potency with mortalities of 90–100% for R. losea and 77·8–100% for A. agrarius. Experimental baits prepared using the manufacturing 0·5% master mix of flocoumafen were palatable to both species.     

The reproductive potential of Heterakis gallinarum in various species of galliform birds: implications for survival of H. gallinarum and Histomonas meleagridis to recent times

The reproductive potential of Heterakis gallinarum was substantially higher in the ring-necked pheasant than in any of the eight other species of galliform birds used on the 67 tests here reported. Pheasants on four tests yielded an average 19·4 times as many eggs that embryonated as were used to infect the birds, while for those on tests with a highly virulent strain of Histomonas meleagridis present the return was 21·1 eggs per egg used. Corresponding returns for chickens were 5·2 and 2·4; for guinea fowl, 9·7 and 1·3; and for turkeys, 1·9 and 0·17. Birds of the other five species gave even poorer returns. Previous studies had indicated that 10–30 times as many heterakid eggs must embryonate as survive to be ingested, under natural conditions. Inasmuch as the traditional host of Heterakis gallinarum must also have been that of the virulent strains of Histomonas meleagridis that have become man's contemporaries, we regard the ring-necked pheasant, or some very close relative, as being the most likely host of these parasites in the late Cenozoic and Recent Eras.     

Ontogeny of critical and prolonged swimming performance for the larvae of six Australian freshwater fish species

Critical (<30 min) and prolonged (>60 min) swimming speeds in laboratory chambers were determined for larvae of six species of Australian freshwater fishes: trout cod Maccullochella macquariensis, Murray cod Maccullochella peelii, golden perch Macquaria ambigua, silver perch Bidyanus bidyanus, carp gudgeon Hypseleotris spp. and Murray River rainbowfish Melanotaenia fluviatilis. Developmental stage (preflexion, flexion, postflexion and metalarva) better explained swimming ability than did length, size or age (days after hatch). Critical speed increased with larval development, and metalarvae were the fastest swimmers for all species. Maccullochella macquariensis larvae had the highest critical [maximum absolute 46·4 cm s^?1 and 44·6 relative body lengths (L_B) s^?1] and prolonged (maximum 15·4 cm s^?1, 15·6 L_B s^?1) swimming speeds and B. bidyanus larvae the lowest critical (minimum 0·1 cm s^?1, 0·3 L_B s^?1) and prolonged swimming speeds (minimum 1·1 cm s^?1, 1·0 L_B s^?1). Prolonged swimming trials determined that the larvae of some species could not swim for 60 min at any speed, whereas the larvae of the best swimming species, M. macquariensis, could swim for 60 min at 44% of the critical speed. The swimming performance of species with precocial life‐history strategies, with well‐developed larvae at hatch, was comparatively better and potentially had greater ability to influence their dispersal by actively swimming than species with altricial life‐history strategies, with poorly developed larvae at hatch.     

Cultivation of Lemna gibba under desert conditions. I: Twelve months of continuous cultivation in open ponds

Duckweed, Lemna gibba, was grown in 12 m² shallow ponds in the Negev desert, during 12 months of continuous cultivation, beginning April 1984. Average monthly growth rates varied with the season of the year. The lowest daily yield, 2·6±0·4 g dry weight m⁻² day⁻¹, was obtained during January. Highest daily yields, 7·9±2·6 g dry weight m⁻² day⁻¹ and 7·0±1·2 g dry weight m⁻² day⁻¹, were obtained during September and May. A 35% decline of the yield was seen during midsummer (July), 4·8±1·2 g dry weight m⁻² day⁻¹. The average rate for the year was 5·15±1·7 g dry weight m⁻² day⁻¹. The protein content of the plants ranged from 30 to 38% per unit dry weight.Growth performance is discussed in relation to the prevailing climatic conditions.     

Differential net food utilization by larvae of Sitophilus oryzae and Sitophilus granarius

The net utilization of a meridic diet by Sitophilus oryzae from the newly hatched larva to the pupa was more efficient compared with that of S. granarius. The artificial diet was highly digestible to both species, but S. oryzae converted 24·1 per cent of the ingested food into body substance compared with 12·4 per cent converted by S. granarius. The mean pupal weight of S. granarius (1·402 mg) was greater than that of S. oryzae (1·012 mg); however, larvae of S. granarius consumed 2·6 times as much food and excreted 8·1 times as much faecal material to obtain that weight. Even though S. granarius consumed the diet at a greater rate, the relative growth rate of S. oryzae was faster. The intracellular symbiotes present in S. oryzae may have a rôle in the species' faster development and more efficient utilization of its food.     

Patterns of nitrogen utilization between the ambrosia beetle Xyleborus dispar and its symbiotic fungus

Some parameters of nitrogen utilization between the ambrosia beetle Xyleborus dispar in mutualistic association with its symbiotic fungus Ambrosiella hartigii, were examined. Qualitative and quantitative analyses of the major nitrogenous excretory products were made on the various life stages of X. dispar. The main nitrogenous product found in excreta and hindguts of beetles, larvae, and pupae, was uric acid (range 7·6–14·8 μg uric acid/beetle). No ninhydrin-positive compounds were located in excreta of the beetles. The concentration of ammonia-nitrogen in the various life stages averaged between 0·70 and 1·13 μg NH₃-N/beetle.Total nitrogen determinations were made on sapwood samples of Malus sylvestris (0·34 ± 0·005% N by dry weight), attacked wood, ‘pre-brood’ (0·31 ± 0·005% N by dry weight), and attacked wood ‘post-brood’ (0·17 ± 0·02% N). Similar determinations of the artificial medium (l-asparagine medium) indicated that a nitrogen requirement of about 0·08–0·1% N by dry weight was necessary before oviposition could occur.Fixation of atmospheric nitrogen by individual X. dispar beetles in vitro was not indicated using the acetylene ethylene reductase method. Proteolytic enzyme activity was not found on examination of diapause beetles, their excreta, larval and pupal excreta, and the ambrosial and mycelial forms of A. hartigii.Comparative concentrations of soluble proteins and free amino acids suggested that fungus in the mycangia was built up from free amino acids of the insects. At the period of emergence, flight, and attack of new hosts, the females were found to have a concentration of soluble proteins more than double that found in the beetles during the remainder of the year. The free amino acids were the lowest values recorded during this period (March–October).     

First data on the nuclear DNA content (Feulgen-positive material) of Perodicticus potto

The nuclear DNA content (Feulgen-positive material) of Perodicticus potto, measured on lymphocytes from six animals of the subspecies edwarsi (Gabon) and potto (Dahomey and Liberia) is quite homogeneous around a mean value of 6·87 ± 0·15 pg. A difference of 1·5% has been found between sexes in each subspecies; the possible relation of this fact to the characteristics of the karyotype is discussed.     

Localization of repetitive and unique DNA sequences neighbouring the rabbit beta-globin gene

The structure of oxymyoglobin has been refined at 1·6 Å resolution, using diffractometer data collected at ?12 °C. The crystallographic R factor is 0·159, and the atomic positions are known to 0·1 Å accuracy in internal segments of the molecule.The iron atom lies 0·22(3) Å from the plane of the porphyrin, 0·25 Å closer than in deoxymyoglobin, and the F helix has moved by a similar amount. Oxygen binds to the iron in a bent, end-on arrangement, with FeOO = 115(5) ° and FeO = 1·83(6) Å. The mean FeN(porphyrin) bond length is 1·95(6) Å, 0·08 Å shorter than in deoxymyoglobin, but the difference is not significant compared to the experimental error. FeN_ε(His8F) is 2·07(6) Å, the same as in model compounds. Movements of the haem, iron, F helix and FG corner on oxygenation are similar to those found in the T-R state transition in haemoglobin, but are smaller in magnitude.     

In vitro synthesis of peritrophic membranes of the blowfly, Calliphora erythrocephala.

Tyrode solution containing added glutamine and Leloup's medium 1 has been used as a basic medium for the in vitro culture of the so-called proventriculus of adult Calliphora erythrocephala to elucidate some of the factors controlling the synthesis of peritrophic membranes (PM) in vitro. The formation rate was chosen as a quantitative criterion for the evaluation of the modifications of the incubation media.After systematic variation of osmolarity, pH, and temperature optimal formation rates were obtained in media with an osmolarity of 320 to 360 mOsmol, a pH of 6·8, and an incubation temperature of 27°C. Under these conditions the average rate of formation was in the modified Tyrode solution 3·0±1·1 mm PM/hr, and in Leloup's medium 3·6±0·8 mm PM/hr. In the modified Tyrode solution the formation of PM was complete after 5 to 7 hr, whereas in Leloup's medium it continued up to 24 hr. The addition of β-ecdysone caused an increase of the formation rate of PM to 4·5 to 5·5 mm PM/hr.The results obtained led to the hypothesis that an osmotically regulated enzyme system could be the limiting factor of the formation rate of peritrophic membranes, i.e. a system which could regulate the internal osmolarity of the formative cells by the interconversion of a bulk polymer and its monomer which are needed for the synthesis of PM.     

Dynamics of the pregnancy cycle in the tsetse Glossina morsitans

A normal pregnancy in tsetse involves the successful integration of larval development with maternal activity. At 25°C, ovulation in Glossina morsitans occurs 1 hr after the previous larviposition, the egg hatches on day 3·8 (1·57 mm length, 0·09 mg dry wt.), ecdysis to second instar occurs on day 4·9 (2·3 mm, 0·30 mg), the third instar cuticle is formed on day 6·8 (4·5 mm, 5·0 mg), and parturition occurs on day 9·0 (6·0 mm, 10·0 mg). Melanization of the in utero third instar follows a regular sequence over a 2 day period. Parturition follows a circadian pattern with a peak 9 hr after lights on (12 hr daily photophase). All instars receive nutriment from the female's milk gland. During early pregnancy the rate of milk synthesis is greater than rate of uptake by the larva, thus causing expansion of the secretory reservoirs. After day 6, the volume of the secretory reservoirs decreases, but as is indicated by nuclear volume and larval growth the rate of synthesis remains high until day 8. Feeding activity of the adult female is maximal on day 1, levels off at 60 per cent up to day 6, and then declines sharply towards the end of pregnancy. Oöcyte development proceeds in phase with larval development and thus minimizes a lag period between successive pregnancies.     

Fine structure and motility of spermatozoa and composition of the seminal plasma in the perch

The fine structure and motility of spermatozoa and the composition of the seminal plasma of the perch Perca fluviatilis are investigated by electron microscopy, computer assisted cell motility analysis (CMA) and biochemical methods. The spermatozoon is asymmetrical as the flagellum inserts mediolateral on the nucleus. It lacks an acrosome, has an ovoid head and a small midpiece with one mitochondrion. Sperm motility–initiated in distilled water (10° C)–is characterized as follows: 85·0 ± 2·7% of the spermatozoa are motile, the main swimming type (10 ± 1 s after motility initiation) is the linear motion (61·4 ± 24·4%) and the average swimming velocity is 122·4 ± 21·9 μm s^–1. When motility is initiated with NaCl, glucose or sucrose solutions of 100 mosmol kg^–1 the percentage of motile spermatozoa and the swimming types are similar as in water, but the swimming velocity (174·0 ± 22·3 μm s^–1) is significantly higher. Motility is inhibited by high osmolality of the diluent: when increasing the osmolality of the saline solutions to 350 mosmol kg^–1 sperm motility is totally suppressed while potassium (10–40 mmol 1^–1) does not affect motility parameters. pH optimum for sperm motility is between pH 7·0 and 8·5. The seminal fluid contains 124·01 ± 21·68 mmol 1^–1 sodium, 10·22 ± 1·11 mmol 1^–1 potassium and 0·72 ± 0·26 mmol 1^–1 calcium. pH is 8·25 ± 0·09, and osmolality 283·90 ± 37·19 mosmol kg^–1. The following organic components were determined: monosaccharides (glucose 63 ± 19 μmol 1^–1, fructose 54 ± 28 μmol 1^–1, galactose 59 ± 25 μmol 1^–1), lipids (cholesterol 5·51 ± 6·42 μmol 1^–1, triglycerides 72 ± l00 μmol l^–1, cholesteryloleate 15–150 μmol 1^–1, phosphatidylcholine 26 · 31 μmol 1^–1, glycolipids 1–10 mg 100 m1^–1), lactate 108 ± 99 μmol 1^–1, hydroxybutyrate 102 ± 99 nmol 1^–1, choline 59 ± 159 μmol 1^–1, protein 344·75 ± 59·06 mg 100m1^–1, enzymes (β-d -glucuronidase l.4 ± 0.7 μmol h^–1 100 ml^–1, protease (caseolytic activity) 1·0 ± 0·6 μmol h^–1 100 ml^–1, alkaline phosphatase 2520·0 ± 861·0 μmol h^–1 100 ml^–1, acid phosphatase 44.0 ± 16.0 μmol h^–1 100 ml^–1, glucose-6-phosphate dehydrogenase 38·9 ± 86·9 μmol h^–1 100 ml^–1, lactate dehydrogenase 134·4 ± 69·6 μmol h^–1 100 ml^–1, butyrylcholine esterase 0·014 ± 0·010 μmol h^–1 100 ml^–1, adenosine triphosphatase 562·8 ± 665·4 μmol h ^–1 100 ml^–1).     

Sequence rearrangements between mitochondrial DNAs of Torulopsis glabrata and Kloeckera africana identified by hybridization with six polypeptide encoding regions from Saccharomyces cerevisiae mitochondrial DNA

Sequences hybridizing to six mitochondrial DNA encoded polypeptide genes of Saccharomyces cerevisiae have been mapped in the 18·9 and 27·1 kbp² circular mitochondrial DNAs from Torulopsis glabrata and Kloeckera africana. With the possible exception of cytochrome oxidase subunit 1 and ATPase subunit 6 genes, no two hybridizable sequences share the same order in the two mtDNAs nor is there any topographical similarity to S. cerevisiae mtDNA apart from the grouping mentioned above. Because sequence rearrangements are prevalent in yeast mitochondrial DNAs we infer that order is not critical for mitochondrial gene expression and that prokaryotic-like operons do not exist. In contrast to S. cerevisiae, the cytochrome b region in T. glabrata and K. africana is confined to 1·46 or 1·58 kbp, respectively, which suggests that intervening sequences in this gene are either small or absent. On the other hand, hybridizable sequences to a 5·2 kbp portion of the S. cerevisiae cytochrome oxidase subunit 1 gene, retaining exons 3 to 7 or 8, span 3 to 4 kbp in the two mtDNAs. In addition an 0·8 to 0·9 kbp intervening sequence is present in each case, which does not hybridize to either exon or intron regions of the S. cerevisiae probe. These results imply that the cytochrome oxidase subunit 1 gene in both mtDNAs has a mosaic organization of coding and noncoding sequences.