Molecular cloning and DNA sequence analysis of genes encoding cytotoxic T lymphocyte-defined HLA-A3 subtypes: the E1 subtype

Influenza-specific cytotoxic T cells restricted by HLA-A3 and allogeneic CTL specific for HLA-A3 recognize differences between serologically indistinguishable HLA-A3 antigens. Previous biochemical studies have indicated that such differential recognition can be explained by alterations in the primary structure of class I heavy chains. Characterization of these sequence differences may therefore identify portions of the class I molecule that form determinants recognized by CTL. In this study, we describe the cloning and sequencing of an HLA-A3 subtype from donor E1 (E1-A3). Cloning of the gene encoding E1-A3 was simplified by determining that a 15.5-kb BamHI fragment contains the complete gene and is characteristic of HLA-A3 and only one other class I gene (HLA-A11). Comparison of the E1-A3 sequence to that of a previously sequenced HLA-A3 gene for exons encoding extracellular class I domains revealed three nucleotide differences. All of these differences were located within a discrete region of exon 3 (encoding the alpha 2 domain) and result in a change of two amino acids, at positions 152 (Glu----Val) and 156 (Leu----Gln). This finding suggests that these amino acids are crucial for the information of a determinant recognized by CTL. Furthermore, the altered nucleotide sequence of E1-A3 is identical to the sequence of the HLA-Aw24 gene for codons 128 to 161. These observations of multiple clustered changes in the E1-A3 subtype (relative to the prototype sequence) and identity of the altered sequence with the sequence of another class I gene support the concept that gene conversion is a primary mechanism for the generation of class I polymorphism.     

Crystallization and preliminary crystallographic data of the Fab fragment of an anti-phenylalanine hydroxylase monoclonal antibody

Two crystal habits, one rod shaped and the other square prismatic, of the Fab fragment of a monoclonal anti-phenylalanine hydroxylase antibody have been grown using the method of vapour phase diffusion against polyethylene glycol 6000. The square prisms diffract to better than 2.8 A, belong to the space group P1 and have unit cell parameters a = 41.8 A, b = 50.3 A, c = 114.7 A, alpha = 97.6 degrees, beta = 91.7 degrees, gamma = 91.0 degrees, while the rod-shaped crystals belong to the space group P212121, have unit cell parameters a = 105.6 A, b = 119.8 A, c = 82.2 A and diffract to 3.5 A resolution.     

Secretory bursts of growth hormone secretion in the dog may be initiated by somatostatin withdrawal

In 28 6-h experiments on 10 conscious resting trained male dogs, plasma growth hormone (GH) was determined at 5-min intervals by radioimmunoassay. For all experiments, the basal GH concentration in plasma was 0.80 +/- 0.06 ng mL-1. In each experiment, 1-3 secretory bursts of GH occurred, raising plasma GH 2.4 to 15.3 times basal concentrations (for all 43 bursts, 6.6 +/- 0.4 times the basal value). Metabolic clearance rates (MCR) and apparent distribution volumes (V) were determined, using stepwise infusions of canine GH. The MCR (3.99 +/- 0.30 mL kg-1 min-1) and V (57.9 +/- 5.5 mL kg-1) were used to transform the GH concentration versus time data into GH secretion rates, using a single compartment approach. Basal GH secretion rates for all 28 experiments were 3.12 +/- 0.24 ng kg-1 min-1. The secretory bursts yield peak GH secretion rates of 9.4 +/- 0.8 times basal secretion and these steep-sloped bursts last 25.1 +/- 1.2 min. Six-hour infusions of 0.15 microgram kg-1 min-1 of somatostatin (SRIF) abolished all secretory bursts but did not lower basal secretion rates. In five of seven SRIF infusion experiments in which samples were taken after the infusion ceased a secretory burst was seen in the hour following cessation of infusion (in four cases within 10 min). These secretory bursts lasted 23.0 +/- 2.9 min and were similar to those seen in control experiments. Infusions of SRIF at 0.05 microgram kg-1 min-1 had no effect. These results imply that during basal GH secretion, a surfeit of SRIF impinges on the somatotrophs, as extra SRIF does not further lower basal secretion. However, during secretory bursts, very little SRIF must be present, as exogenous SRIF blocks these bursts. The bursts are similar in duration to overshoots provoked in perifused dispersed rat somatotrophs by removal of an SRIF signal. It seems likely that their cause in vivo is similar. (All values are means +/- SEM.)     

Feedback suppression of ACTH secretion by cortisol in dogs: lags after large signals equal those following very small signals

Previously, low stepwise infusions of cortisol in resting adrenalectomized dogs (plateaux less than or equal to 6 micrograms/dL) were shown to reduce ACTH secretion only after 20 min. In the present study, large, steep-sloped cortisol signals were used to try to evoke faster feedback. Adrenalectomized male mongrel dogs were maintained on exogenous steroids until 48 h before the experiment. Of the 23 experiments on 15 dogs (under light pentobarbital anesthesia), 12 were on resting dogs, 7 on dogs stressed by variable insulin infusion (keeping plasma glucose at 18-40 mg/dL), and 4 stressed as above but with 4 h of low cortisol infusion (plasma congruent to 5 micrograms/dL) before applying the feedback signal. After a 50-min control period, a 30-min feedback period was initiated by one of two i.v. cortisol signals: (a) injection of 0.3 mg/kg or (b) infusion of 46 micrograms kg-1 min-1. Both raised plasma cortisol above physiological limits (within 2 and 6 min, respectively). In each experiment, 23 timed venous blood samples were assayed for plasma ACTH and cortisol. ACTH secretion rates were calculated continuously using a validated single-compartment method. Results from both types of cortisol signals were indistinguishable, and were thus pooled. In the unstressed dogs, control-period ACTH secretion of 0.97 +/- 0.12 mU kg-1 min-1 showed no significant decline due to the feedback signal for 20.3 +/- 1.4 min.(ABSTRACT TRUNCATED AT 250 WORDS)     

Effect of pinealectomy on seasonal changes in antler growth and concentrations of testosterone and prolactin in white-tailed deer

A 2-year study was conducted to determine under controlled conditions the role of the pineal gland in regulating the seasonal changes in antler growth and reproduction of male white-tailed deer. Blood samples were drawn from 6 pinealectomized (PX) and 18 control (C) deer at intervals of 2 weeks and analyzed for testosterone (T) and prolactin (Prl). Relative scrotal circumference and main beam antler length were recorded. Relative scrotal circumference was similar in PX and C groups, but the normal pattern was delayed 1 to 3 months in the PX deer relative to the C deer. The mean dates of beginning antler growth, velvet shedding, antler casting and pelage changes were significantly later in both years for PX deer than in C deer. Testosterone concentrations peaked 1 month later in the PX deer than in the C deer for both yearling and 2-year-old deer. Prl concentrations in C deer, but not in PX deer, were correlated highly with day length, and the PX deer were delayed relative to the C deer in showing the normal Prl pattern. Increasing levels of Prl in both groups coincided with beginning antler growth in both years. These results indicate that the pineal gland does not originate the seasonal cycles of male white-tailed deer but may synchronize cycles among individual deer, and regulate the circannual rhythm of Prl concentrations which may in turn influence other hormonal cycles.     

The relative role of stomata in transpiration and assimilation

Summary The ways in which transpiration and assimilation depend on stomatal aperture are compared. It is shown that transpiration and assimilation are equally sensitive to change of stomatal aperture when the internal resistance to assimilation is equal to an effective resistance to evaporation which exists because of the coupling of heat and vapour exchanges between leaf and atmosphere. Generally the ratio of transpiration to assimilation changes with stomatal aperture in a manner which is determined by the relative magnitude of these resistances and on temperature. Some possible implications in relation to the optimal behaviour of stomata are discussed.Work done while J.H.T. held a New Zealand D.S.I.R. Fellowship.     

Probing by aphids in the leaf tissues of resistant and susceptible sugar beet

The probing of Aphis fabae and Myzus persicae in the leaves of sugar beet with inherited resistance or susceptibility to aphids was studied by microscopic examination of samples of whole leaves, prepared after 48 h exposure to adult aphids at approximately three aphids cm^-2.The density of saliva stylet-sheaths left by the aphids (cm^-2) and the proportion reaching phloem differed between sugar beet stocks and were inversely associated. Differences in resistance between stocks could not, however, be related directly to either. All beet stocks examined were probed freely. Seasonal differences in sugar beet grown in the glasshouse affected the proportion of sheaths reaching the phloem, but the differences between beet stocks were similar at all times.The densities of sheaths left by different clones of M. persicae corresponded with the aphids' response to sugar beet as a host plant. Among aphid clones which readily colonize sugar beet, the densities of stylet sheaths which reached phloem suggested that the adults of both A. fabae and M. persicae gained sufficient access to sieve tubes to satisfy their nutritional needs. The phloem of sugar beet from the glasshouse was always within the estimated maximum depth to which the aphids probe; but, in leaves from the field, it appeared that the phloem might be inaccessible to young M. persicae in the sugar beet crop during late summer.

---

Zusammenfassung Das Proben von Aphis fabae und Myzus persicae in Blättern von Zuckerrüben mit erblicher Blattlausresistenz bzw.-anfälligkeit wurde untersucht durch mikroskopische Durchmusterung von Speichelscheiden in Proben von ganzen Blatt. Rübenblätter wurden mit genähert drei adulten Läusen cm^-2 besetzt und nach 48 Stunden quergeschnittene Streifen der Blätter in Alkohol fixiert, gefärbt und mit der Unterseite nach oben auf Objektträgern eingeschlossen.23890 Speichelscheiden wurden registriert. Die Dichte der Scheiden von M. persicae (cm^-2) und der Anteil der das Phloem erreichenden Scheiden (SRP) unterschieden sich signifikant zwischen den Rübenstämmen. Bei A. fabae ergaben sich entsprechende, aber nicht gesicherte Unterschiede. Scheidendichte und Prozentsatz SRP waren gegenläufig, zwei Rübenstämme zeigten eine hohe Scheidendichte, zwei andere hatten weniger Scheiden, aber einen höheren Prozentsatz SRP. Diese Gruppierung der Stämme korrespondierte aber nicht mit ihrer Blattlausresistenz. Aus der Scheidendichte ergab sich, dass M. persicae und A. fabae auf allen geprüften Rübenstämmen, resistenten und anfälligen, unbehindert probten, so dass jede Laus das Phloem durchschnittlich etwa viermal am Tag erreichte. Ein Klon von M. persicae, der sich an Rüben nicht entwickelt, hinterliess weniger Scheiden in den Blättern aller Stämme.Der Anteil von SRP war bei Prüfungen im März grösser als im November. Dieser Unterschied war besonders deutlich bei Scheiden von Larven, die im übrigen zu allen Zeiten das Phloem weniger oft erreichten als ihre Eltern. Messungen des Abstandes von der unteren Blattfläche zum Phloem ergaben, dass das Phloem den Läusen in Gewächshaus-Zuckerrüben immer zugänglich war. M. persicae-Larven konnten jedoch in Blättern von Freilandrüben das Phloem nicht erreichen.

     

Fate of corticotrophins in an isolated adrenal-cell bioassay and decrease of peptide breakdown by cell purification

1. The fate of corticotrophins in a trypsin-dispersed rat adrenal-cell assay system was investigated with a view to establishing whether differences in the rate of inactivation might contribute to potency differences observed between analogues. 2. Corticotrophin-(1-24)-tetracosapeptide and to a lesser extent synthetic 1-39 corticotrophins were found to be inactivated during incubation with cell suspension. 3. Peptide fragments were isolated by using [[(3)H(2)]Tyr(23)]corticotrophin-(1-24)- tetracosapeptide as a marker. The fragments indicate a peptidase with a predominantly tryptic specificity. 4. The peptidase is present in the extracellular fluid and is released from cells when they are damaged. 5. Cells were fractionated on an albumin gradient. Cells from the zona fasciculata and the zona intermedia or reticularis were present in fractions which produced fluorogenic steroids in response to corticotrophin. 6. Purification of the cells by centrifugation through albumin decreased degradation by peptidases, so that if the assay is carried out with a dilute suspension of purified cells peptide breakdown should not affect the observed potencies of adrenocorticotrophin analogues. 7. No binding of [[(3)H(2)]Tyr(23)]corticotrophin-(1-24)- tetracosapeptide to cells could be detected at low concentrations of the peptide. This indicated that less than 120 receptors/cell are occupied during stimulation by a dose that would elicit approx. 80% of the maximal response.     

The Influence of Morphology on Prognosis in Acute Leukemia

The presence of definite cytoplasmic granulation in at least some of the malignant cells was used as the sole criterion to separate 156 patients with acute leukemia into two groups: 110 with myeloblastic (AML), and 46 with lymphoblastic or stem cell leukemia (ALL). The median survival from the onset of symptoms in patients with AML was 20 weeks, and those with ALL 37 weeks. The difference in survival in these two groups is much greater for patients under the age of 25 than for those over the age of 25.