AN AUTORADIOGRAPHIC STUDY OF THE 3H-URIDINE AND 3H-THYMIDINE INCORPORATION IN THE REGENERATING MOUSE LIVER

An autoradiographic study was made of the ³H-uridine incorporation into RNA and DNA in nucleus and cytoplasm of parenchymal cells in the regenerating liver of the mouse after a pulse time of 2 hr. After a decreased uptake of precursor into the parenchymal nucleus during the first 6 hr compared with the normal value, incorporation increased and was maximal at 36 hr; normal values were restored at 72 hr. The cytoplasmic labelling, after an initial small decrease, reached a maximum at 12 hr; this changed to normal 48 hr after hepatectomy. RNase-digestion of the liver sections left a small incorporation in both nucleus and cytoplasm: presumably DNA. This incorporation is maximal at 12 hr over the nucleus and at 24 hr over the cytoplasm. After a 2 hr pulse of ³H-thymidine, there was a marked uptake of the precursor into DNA about 24 hr after hepatectomy. This was maximal at 48 hr and reached normal values at 72 hr. A small amount of incorporation of ³H-thymidine into DNA was seen immediately after the operation, and this population of weakly labelled nuclei was still rather large 72 hr later.     

BIOCHEMICAL EFFECTS OF THYROID DEFICIENCY ON THE DEVELOPING BRAIN

Abstract— The effects of neonatal thyroidectomy on some constituents of the cerebrum, cerebellum and liver of the rat have been studied during the first 7 weeks of life. In the normal rat between the 6th and 14th post-natal days the RNA content per unit of DNA in the brain increased by 70 per cent. Although the brain continued to grow from the 14th to the 35th day, the amount of RNA relative to DNA decreased by about 20 per cent. The ratio of protein to DNA increased during the whole period studied and in the cerebral cortex it was more than trebled between the age of 6 and 35 days. The growth of the cerebellum extended over a longer period than that of the cerebrum, its weight increasing by 88 per cent between the ages of 14 and 35 days as compared with a cerebral increase of 34 per cent. The DNA content showed a 50 per cent increase during this period. Qualitatively these maturational changes were not affected by neonatal thyroidectomy. Quantitative changes, which applied equally to the cerebral cortex and brain as a whole, were observed. At the age of 35 days, the weights of the cerebral hemispheres and cerebellum were reduced by thyroidectomy by 20 per cent; the overall DNA content per organ did not change, but the amounts of protein and RNA relative to DNA decreased significantly. It is therefore inferred that thyroid deficiency affects the size of the cells in brain and cerebellum rather than their total number. Conversely, the cell population of the liver was only a quarter of that in the control. There was a small but significant decrease in the hepatic protein and RNA content in the hypothyroid animal. The activities of the following enzymes which served as markers for subcellular fractions in homogenates of cerebral cortex were determined: lactate dehydrogenase for the supernatant, glutamate dehydrogenase for the mitochondrial and glutamate decarboxylase for the synaptosomal fractions. When the activities were expressed on a fresh weight basis a significant decrease by comparison with the control values was observed only in the case of glutamate decarboxylase (—15 per cent at the age of 17–32 days); when the activities were based on DNA content all values were reduced, probably as a result of the general decrease in cell size. Pyrimidine metabolism of brain and liver, studied after the administration of [6-¹⁴C]-orotic acid, was not affected in either tissue by neonatal thyroidectomy. A small but significant reduction in the incorporation of labelled pyrimidine nucleotides in liver RNA was observed, but no significant decrease in the incorporation in cerebral RNA was found in the hypothyroid rats.     

PUROMYCIN-INDUCED NECROSIS OF CRYPT CELLS OF THE SMALL INTESTINE OF MOUSE

Chemical and radioautographic analysis of the small intestine of mice injected intraperitoneally with puromycin revealed an immediate decrease of precursor incorporation into DNA and protein and a delayed decrease of precursor incorporation into RNA. In addition to this decrease of precursor incorporation, damage to the crypt cells, but not to the cells of the villus of the small intestine, was observed. Further examination of other dividing cells (spleen) and nondividing cells (liver and heart) of these mice showed again that only cells of actively dividing tissues were damaged. The metabolic inhibitors actinomycin D, cytosine arabinoside, actidione, and puromycin aminonucleoside were used in an attempt to clarify the mechanism of cell damage by puromycin. The results showed that there was no clear correlation between cell necrosis and the pattern of inhibition of synthesis of DNA, RNA, or protein.     

饥饿和再投喂对草鱼鱼种生物化学组成的影响

分析了饥饿１５天和再投喂２１天的草鱼鱼种肝脏和肌肉生物化学组成的变化，结果表明：（１）饥饿降低白肌ＲＮＡ／ＤＮＡ比值，蛋白质含量和肝脏ＲＮＡ／ＤＮＡ比值，使肝脏蛋白质含量升高，再投喂后，肝脏ＲＮＡ／ＤＮＡ比值，蛋白质含量和白蛋白质含量均恢复至正常投喂组水平，白肌ＲＮＡ／ＤＮＡ比值升高并显著高于正常投喂组水平；（２）饥饿状态下，肝脏和肌肉的脂类含量降低，水含量升高，再投喂后，肝脏和肌肉的脂类含量升高     

短期饥饿和再投喂对岩原鲤仔鱼生存生长以及RNA/DNA和RNA/蛋白质比率的影响(英文)

研究通过对岩原鲤仔鱼在饥饿和再投喂条件下其生存、生长率、RNA/DNA和RNA/蛋白质比率的测定,评估了仔鱼对饥饿的耐受能力和恢复能力。在(19.5±0.5)℃水温下,将岀膜后第16天的岩原鲤仔鱼随机分成6个组:1个持续投饲对照组,实验组分别禁食1、2、3、4、5d后再投喂,实验共进行10d。每天分别从各组取9尾鱼测定体重、体长、RNA、DNA、蛋白质含量。实验结果显示,饥饿处理组仔鱼存活率和以上各项生长指标均随饥饿时间的增加而下降,在恢复投喂后均表现不同程度的补偿生长,其中饥饿1、2、3d的仔鱼在恢复投喂后显示出完全补偿生长,几乎弥补了饥饿所产生的影响,平均终体重与对照组比较无显著差异。饥饿4、5d的仔鱼显示部分补偿生长,恢复投喂只少量减轻了饥饿的影响,平均终体重与对照组相比存在显著差异。饥饿1、2、3d的仔鱼和4、5d的仔鱼在恢复投喂后分别需要1—2d和4d时间才能达到与对照组无显著差异水平。仔鱼生长率变动范围从0.59%到8.00%WW/day,仔鱼RNA/DNA比率、RNA/蛋白质比率与生长率的回归方程为:GR=3.63RNA/DNA 1.74(R2=0.80)和GR=120.14RNA/Protein 2.33(R2=0.31),两种比率均与生长率呈显著线性相关,RNA/DNA比率对生长变化的拟合度更好。结果表明,仔鱼阶段食物缺乏很可能是影响岩原鲤仔鱼存活、生长的主要因素。RNA/DNA更适合作为评定岩原鲤仔鱼营养条件和生长的指标。     

端粒酶RNA反义基因对肝癌细胞的影响

用RT-PCR的方法钓取端粒酶RNA基因的cDNA,并将其反向插入到逆转录病毒载体pLNCX上,构建hTR基因的反义表达质粒。将质粒经脂质体介导转染人肝癌SMMG-7721细胞中表达。结果表明hTR反义基因的表达有效地封闭或抑制肝癌细胞的端粒酶活性,抑制细胞的生长和增殖,延长细胞的倍增时间并促进细胞凋亡。     

IMPAIRMENT OF GROWTH AND DEVELOPMENT OF THE RAT BRAIN BY HYPEROXIA AT ATMOSPHERIC PRESSURE

Abstract— The continuous exposure of newborn rats to 70–80 per cent oxygen at atmospheric pressure throughout the iirst 9 days of life significantly inhibited the growth of the brain which normally occurs during this period of life. The accumulations of DNA, RNA, total protein, and proteolipid protein which accompany brain growth during this period were all approximately proportionately depressed by the oxygen-enriched atmosphere. RNA/DNA and protein/DNA ratios were unaffected. The increase in brain mass in the first week of life reflects mainly cell proliferation, and since the decreased DNA accumulation occurred with no changes in RNA/DNA and protein/DNA ratios, we conclude that the effect of oxygen was to inhibit cellular division. We estimate that the oxygen exposure caused an approximately 7 per cent deficit in the cell population of the brain. These results indicate that the use of elevated concentrations of oxygen may have serious deleterious effects on the growth and development of the brain.     

Mitochondria isolated from liver contain the essential factors required for RNA/DNA oligonucleotide-targeted gene repair

Chimeric RNA/DNA oligonucleotides (ONs) have been used successfully for site-specific modifications of episomal and chromosomal DNA in eukaryotic cells. We explored the possibility of applying this technique to mitochondrial DNA, as single-nucleotide defects in this genome are associated with a series of human diseases. Therefore, we determined whether mitochondria possess the enzymatic machinery for chimeric ON-mediated DNA alterations. We utilized an in vitro DNA repair assay and an Escherichia coli readout system with mutagenized plasmids carrying point mutations in antibiotic resistance genes. RNA/DNA ONs were designed to correct the defects and restore kanamycin and tetracyclin resistance. Using this system, we demonstrated that extracts from highly purified rat liver mitochondria possess the essential enzymatic activity to mediate precise single-nucleotide changes. Interestingly, the frequency of gene conversion was similar in both mitochondrial and nuclear extracts, as well as from quiescent and regenerating liver. The results indicate that mitochondria contain the machinery required for repair of genomic single-point mutations, and suggest that RNA/DNA ONs may provide a novel approach to the treatment of certain mitochondrial-based diseases.     

烟草愈伤组织继代培养与分化期间核酸代谢的比较研究

柳叶烟草愈伤组织在分化和芽原基形成期间,DNA 和RNA 含量均高于继代培养物;在芽原基形成后和幼芽生长期间(12天以后),DNA和RNA 含量持续上升,而同期继代培养物巳进入生长静止期,DNA 和RNA 含量基本不变或略有下降。根据RNA 电泳结果还进一步分析了两种愈伤组织培养物各RNA 组分变化与总RNA 含量变化的关系。分化培养物在芽原基形成时有明显升高的RNase 活性峰和持续上升的RNA 合成速率;而此时期继代培养物的RNase 活性及RNA 合成能力均较低;分化愈伤组织的DNA 合成速率在幼芽生长期间仍维持上升趋势,且显著高于同期继代愈伤组织的合成速率。这些结果表明,烟草愈伤组织分化培养物比继代培养物有更旺盛的核酸代谢能力。     

THE EFFECT OF CORTISONE ON DNA CONTENT OF RAT HEPATOCYTES

Rats were treated with cortisone, x-radiation, and both agents in combination, and the effect noted on the DNA content of hepatocytes. Nuclei were enumerated both in whole liver homogenates and following isolation. The incorporation of P³² into DNA was also studied in relation to these agents. The following observations were made:— 1.The DNA content of nuclei fell both during cortisone administration and following x-radiation. In the former instance, the fall was progressive with continuing administration of hormone; in the latter instance, there was a return to normal 5 days after radiation. 2. Cortisone administration to x-radiated rats caused a fall in DNA/nucleus and prevented the return to normal at 5 days. 3. There was no evidence that the effects of cortisone and x-rays were additive in reducing DNA/nucleus. 4. These data indicate an alteration in DNA/nucleus, but simple changes in ploidy cannot be excluded. Either explanation requires that the agents used affect the DNA of non-regenerating nuclei. 5. Cortisone interfered with the incorporation of P³² into the DNA of regenerating liver. Only a small effect on DNA synthesis in resting liver was observed with cortisone or x-radiation. 6. DNA content of nuclei returned to normal 5 days after x-radiation and 3 days after discontinuance of cortisone. Slight increase in the incorporation of P³² by DNA was observed during recovery phases. 7. The hypothesis is proposed that the apparent losses and increases in DNA/nucleus were due to depolymerization and repolymerization of DNA. Following x-radiation and/or cortisone administration, it is proposed that some DNA is depolymerized and becomes cold acid-soluble and dissociated from organized chromatin. Later, conditions are such that this degraded DNA is repolymerized. 8. These data might be interpreted to indicate that a portion of the DNA is not essential to cell integrity; alternatively, there may be two or more species of DNA, one of which is more readily affected by the agents investigated in the present report.     

云南油杉原胚发育过程中组织化学的变化

应用组织化学方法对云南油杉(Keteleeria evelyniana Mast)受精前后,原胚及幼胚形成早期细胞内的DNA、RNA、碱性蛋白质,酸性蛋白质及多糖物质进行了观察。结果表明,DNA在卵核受精前后为孚尔根弱正反应。在原胚及早期幼胚发育过程中,胚原细胞核DNA含量恢复正常,RNA及酸性蛋白质含量均较丰富,特别是在胚原细胞内。新细胞质中碱性蛋白质呈负反应,而DNA、RNA、酸性蛋白质及多糖物质均呈现正反应。     

THE ISOLATION OF CELL NUCLEI FROM RAT BRAIN

A method for preparing highly pure cell nuclei from adult rat brain, using both differential and isopycnic centrifugation in sucrose media, is described. The morphology of these preparations was examined by both phase contrast and electron microscopy. The isolated nuclei retained many aspects of their in situ morphology; in particular, the nuclear envelope was double layered and interrupted by pore-like discontinuities, and the nucleoli consisted of irregular masses of densely packed granules. Analyses of these nuclear preparations for cytochrome oxidase and cholinesterase activity, as well as RNA/DNA ratio, indicated minimal contamination with mitochondria and microsomes. Problems involving the homogenization technique, choice of ionic conditions in the homogenization medium, and choice of optimal density of the sucrose solution used for the final purification of nuclei are discussed. Results of application of the technique to isolation of adult rat liver nuclei are also reported.     

FRACTIONATION OF THE RNA COMPONENTS OF RAT BRAIN POLYSOMES

Abstract— The incorporation in vivo of [³H]uridine into the RNA isolated from the free polyribosomes of rat cerebral cortex was studied. Sedimentation in sucrose gradients showed that initially (at times less than 60 min after injection of precursor) the label was associated with a heterodisperse species, while at longer times there was an increased coincidence of label with stable rRNA. Further fractionation was accomplished by means of differential extraction with phenol and analysis on polyacrylamide-agarose gels. Most of the rapidly labelled RNA was concentrated in a fraction obtained at pH 8-3 and 40°C. The base composition of this fraction differed greatly from that of rRNA, preribosomal RNA and DNA. Analysis by electrophoresis on polyacrylamide-agarose gels showed it to be composed of several distinct species in addition to residual 18 and 28S rRNA. Most of the latter was concentrated in a fraction extracted at pH 60 at 0°C.     

饲料蛋白质水平对洛氏鱥生长、非特异性免疫及蛋白质合成的影响

为了研究饲料蛋白质水平对洛氏鱥(Rhynchocypris lagowskii Dybowski)生长、非特异性免疫及蛋白质合成的影响, 以洛氏鱥幼鱼[(6.98±0.01) g/尾]为研究对象, 以鱼粉、棉粕、豆粕及菜粕为蛋白源, 配制成蛋白质水平为24.98%、30. 02%、34.99%、40.01%和44.98%的5种等能、等脂肪的配合饲料, 进行为期8周的饲养试验。结果表明, 在试验条件下, 随着饲料蛋白质水平的升高, 洛氏鱥的终末体质量、特定生长率、增重率均呈先升高后降低的趋势, 其中34.99%和40.01%组洛氏鱥的终末体质量、特定生长率及增重率显著高于24.98%组(P<0.05); 随着饲料蛋白质水平的升高, 洛氏鱥饲料效率和蛋白质效率呈先升高后降低的趋势, 其中40.01%组洛氏鱥饲料效率和蛋白质效率显著高于24.98%组(P<0.05), 但与30.01%、34.99%和40.01%组差异不显著(P>0.05)。通过折线回归分析得出, 饲料蛋白质水平为35.89%时, 洛氏鱥的特定生长率最高; 饲料蛋白质水平为36.11%时, 洛氏鱥饲料效率最高。洛氏鱥肌肉中粗蛋白质含量随饲料蛋白质水平的升高呈先上升后下降趋势, 其中, 40.01%组洛氏鱥肌肉中粗蛋白质含量显著高于24.98%、30.02%、34.99%和44.98%组(P<0.05); 而洛氏鱥肌肉中粗脂肪含量随饲料蛋白质水平的升高呈先下降后上升趋势, 其中, 40.01%组显著低于24.98%、30.02%和34.99%组(P<0.05), 但与44.98%组差异不显著(P>0.05)。洛氏鱥肝胰脏的碱性磷酸酶(AKP)、酸性磷酸酶(ACP)、超氧化物歧化酶(SOD)和溶菌酶(LZM)活性随饲料蛋白质水平的升高呈先上升后下降的趋势, 其中40.01%组洛氏鱥AKP、ACP、SOD和LZM活性显著高于24.98%、30.02%、34.99%和44.98%组(P<0.05); 洛氏鱥白肌中RNA含量和RNA/DNA比值随饲料蛋白质水平的升高呈先升高后降低的趋势, 其中40.01%组洛氏鱥白肌中RNA含量和RNA/DNA显著高于24.98%、30.02%、34.99%和44.98% (P<0.05)。通过折线模型回归分析可知饲料蛋白质水平为36.10%时, 洛氏鱥白肌中RNA含量最高; 饲料蛋白质水平为35.91%时, 洛氏鱥白肌中RNA/DNA比率最高。在洛氏鱥配合饲料中, 最适宜蛋白质需求水平为34.99%—40.01%。     

RNA SYNTHESIS IN THE DIFFERENT PHASES OF CELL CYCLE OF CHICK EMBRYO CELLS

RNA synthesis was studied at different phases of the cell cycle of chick embryo fibroblasts, which were synchronized by medium replacement in the confluent phase. The synthesis of DNA started at 4 hr and continued for 8 hr. RNA synthesis increased with time after medium change. The ratio of total amount of radioactivity in nuclear RNA prepared at 0, 2 and 8 hr was 1.0:1.03:5.05. The distribution of radioactive RNA in the sedimentation pattern was similar, showing remarkable incorporation in 45S region of ribosomal precursor RNA. The base composition of newly synthesized RNA, however, varied at different time intervals after medium replacement. Even within the G₁ phase, the molar percentage of G and C was quite different. Treatment with actinomycin D at a concentration of 0.02 μg/ml for 1 hr specifically inhibited ribosomal RNA synthesis. At 2 hr after medium change, ribosomal and AU-rich RNA including larger than 28S were synthesized in about equal amounts.     

REGULATION OF GROWTH PROCESSES DURING THE CELL CYCLE OF THE CHLOROCOCCAL ALGA SCENEDESMUS QUADRICAUDA UNDER A DNA REPLICATION BLOCK

The kinetics of two growth parameters (total RNA and total protein accumulation) was followed in synchronized cultures of the chlorococcal alga Scenedesmus quadricauda ( Turp.) Bréb. under conditions of inhibited DNA replication in the presence of 5-fluorodeoxyuridine (25 mg.L^-1). In the control culture, growth processes occurred in several steps with a decreasing rate of accumulation of RNA and protein amount approximately at each doubled value of the preceding step. Oscillations in the rate of growth processes in the control culture were temporally related to the initiation of individual reproductive steps. At each doubling, the cell became committed to triggering a sequence of reproductive processes, starting with DNA replication and ending with protoplast fission. Three commitment points were attained in the control culture and, consequently, three replication rounds of DNA followed by three nuclear divisions and three protoplast fissions occurred during one cell cycle. If 5-fluorodeoxyuridine (FdUrd) was added at the beginning of the cell cycle, no reproductive processes occurred, and the cells remained uninuclear with one genome and did not divide. RNA accumulation did not seem to be affected by the presence of FdUrd for at least one cell cycle, and three or four doublings in the amount of RNA occurred during this period. Protein accumulation was even more independent of reproductive processes in the cell and continued for a period of about two or three cell cycles, attaining six doublings at the end of this period. Therefore, oscillations in the rate of protein or RNA accumulation remained even if reproductive processes were inhibited .     

INFLUENCE OF AGE ON THE INCORPORATION OF [14C]GLYCINE INTO PROTEIN IN CHICKEN PERIPHERAL NERVE

Abstract—

• 1 The conditions for incorporation of [¹⁴C]glycine in vitro into proteins in the sciatic nerve of chickens have been studied and found to be similar to those of rat nerve.
• 2 Its incorporation decreases, however, linearly with age.
• 3 The content of RNA and of DNA of peripheral nerve and the RNA/DNA ratio alter linearly with age.
• 4 There is also a linear relationship between the specific radioactivity of the protein extract and the RNA content of the nerve.
• 5 There is a linear decline with age in the specific radioactivity of the protein fraction when expressed against the DNA content.
• 6 A linear relationship exists between the logarithm of the specific radioactivity and the length of the femur.

     

Comparative study on the effects of thyroxine on protein, RNA and DNA contents of liver of different vertebrates at different stages of life

The relative responsiveness of different vertebrates (mammals, amphibia, and fish) at different stages of life to thyroxine (T4) with respect to protein and nucleic acids contents of liver has been studied. The control growing rat, toad, and Lata fish showed a gradual rise in the protein content of liver with the advancement of age. The rat liver RNA reached a maximum level at the 15th d (immature stage) of life and this level was maintained in 30 (juvenile) and 60th d (adult) of life. In the toad, no significant difference in liver RNA was observed with age. Fish liver, however, showed more RNA in juvenile stage than that in immature stage; no such difference was observed in between juvenile and adult stages of life. In normal growing rat, the liver DNA was found to be reduced in juvenile stage from that of immature stage. But in adult stage, the level of DNA was more or less at the same level as that of immature stage of the animals. Fish liver DNA did not exhibit any change with age. But in the toad, the progress of the stages of life was associated with the enhancement of liver DNA. Administration of T4 for 5 consecutive d caused an increase in protein, RNA and DNA contents of liver of rat, toad and Lata fish of different age groups excepting liver DNA in adult toad and fish. The dose of 1 microgram of T4 per g produced maximum effects in these animals. The T4-induced percentage increase in the amount of liver DNA was maximum in immature stage of life; this was followed by an increase in RNA and then by protein. In juvenile stage of these animals, RNA shows maximum increase followed by DNA and/or protein; and in adult stage, the rate of percentage increase in liver RNA was maximum followed by protein and DNA. The dose-response relationship between rat, toad, and Lata fish after T4 treatment (1 microgram/g) revealed that the poikilothermic vertebrates (toad and Lata fish) were more responsive than homoiotherm (rat) so far as the T4-induced increase in liver protein, RNA, and DNA are concerned.