Time line of inventions..China 9th century AD

Gunpowder, also known since in the late 19th century as black powder, was the first chemical explosive and the only one known until the mid 1800s.^[2] It is a mixture of sulfur, charcoal, and potassium nitrate (saltpetre) - with the sulfur and charcoal acting as fuels, while the saltpeter works as an oxidizer.^[3]Because of its burning properties and the amount of heat and gas volume that it generates, gunpowder has been widely used as a propellant in firearms and as a pyrotechnic composition in fireworks.

Gunpowder was, according to prevailing academic consensus, discovered in the 9th century in China, attributed to Chinese alchemists searching for an elixir of immortality.^[4] This discovery led to the invention of fireworks and the earliest gunpowder weapons in China. In the centuries following the Chinese discovery, gunpowder weapons began appearing in the Arab world, Europe, and India. The consensus is that this was spread from China, through the Middle East, and then into Europe,^[5] although there remains some dispute over the amount of Chinese influence on later advancements in gunpowder technology.^{[citation needed]}

Gunpowder is classified as a low explosive because of its relatively slow decomposition rate and consequently low brisance. Low explosives deflagrate at subsonic speeds, whereas high explosives detonate, producing a supersonic wave. Ignition of the powder packed behind a bullet must generate enough pressure to force it from the muzzle at high speed, but not enough to rupture the gun barrel. Gunpowder is thus less suitable for shattering rock or fortifications. Gunpowder was widely used to fill artillery shells and in mining and civil engineering to blast rock roughly until the 2nd half of the 19th century, when the first high explosives (nitro-explosives) were discovered. Gunpowder is no longer used in modern explosive military warheads, nor is it used as main explosive in mining operations due to its cost relative to that of newer alternatives like ANFO.^[6]

Black powder for muzzleloading rifles and pistols in FFFG granulation size. Coin(diameter 24 mm) for comparison.

The Nobel Prize in Physiology or Medicine 2006..Wikipedia

The Nobel Prize in Physiology or Medicine 2006

Andrew Z. Fire, Craig C. Mello

The Nobel Prize in Physiology or Medicine 2006

Photo: L. Cicero

Photo: J. Mottern

Andrew Z. Fire

Craig C. Mello

The Nobel Prize in Physiology or Medicine 2006 was awarded jointly to Andrew Z. Fire and Craig C. Mello "for their discovery of RNA interference

Andrew Zachary Fire
Born	April 27, 1959 (age 52) Palo Alto, California
Residence	Stanford, California
Nationality	American
Fields	Biologist
Institutions	Johns Hopkins University Stanford University
Alma mater	University of California, Berkeley Massachusetts Institute of Technology
Doctoral advisor	Phillip Allen Sharp
Known for	RNA interference
Notable awards	Nobel Prize in Physiology or Medicine (2006)

Small interfering RNA (siRNA), sometimes known as short interfering RNA or silencing RNA, is a class of double-stranded RNAmolecules, 20-25 nucleotides in length, that play a variety of roles in biology. The most notable role of siRNA is its involvement in the RNA interference (RNAi) pathway, where it interferes with the expression of a specific gene. In addition to its role in the RNAi pathway, siRNA also acts in RNAi-related pathways, e.g., as an antiviral mechanism or in shaping the chromatin structure of a genome; the complexity of these pathways is only now being elucidated.

siRNAs were first discovered by David Baulcombe's group at the Sainsbury Laboratory in Norwich, England, as part of post-transcriptional gene silencing (PTGS) in plants. The group published their findings in Science in a 1999 paper titled "A species of small antisense RNA in posttranscriptional gene silencing in plants".^[1] Shortly thereafter, in 2001, synthetic siRNAs were shown to be able to induce RNAi in mammalian cells by Thomas Tuschl, and colleagues in a paper published in Nature.^[2] This discovery led to a surge in interest in harnessing RNAi for biomedical research and drug development.

Mediating RNA interference in cultured mammalian cells.

RNA is an acronym for ribonucleic acid, a nucleic acid. Many different kinds are now known.^[1]

The main function of RNA is to carry information of amino acid sequence from the genes to where proteins are assembled on ribosomes in the cytoplasm. This is done by messenger RNA (mRNA). The sequence of base pairs is transcribed from DNA by an enzyme called RNA polymerase and is reformed in the mRNA. Then the mRNA moves from the nucleus to the ribosomes in the cytoplasm to form proteins. The mRNA translates the sequence of base pairs into a sequence of amino acids to form proteins. This process is called translation.

RNA is physically different to DNA: DNA contains two intercoiled strands whereas mRNA only contains one single strand. RNA also contains different bases to DNA. It contains:

(A) Adenine (G) Guanine (C) Cytosine (U) Uracil

The first three bases are also found in DNA, but Uracil replaces Thymine as a complement to Adenine.

RNA also contains ribose as opposed to deoxyribose found in DNA. These differences result in RNA being chemically more reactive than DNA. This makes it the more suitable molecule to take part in cell reactions.

RNA is the carrier of genetic information in certain viruses, especially the retroviruses like the HIV virus. This is the only exception to the general rule that DNA is the hereditary substance.

Types of RNA.

Non-coding RNAs

Two kinds of non-coding RNAs help in the process of building proteins in the cell. They transfer RNA (tRNA) and ribosomal RNA (rRNA).

[change]tRNA

Transfer RNA (tRNA) is a short molecule of about 80 nucleotides which carries a specific amino acid to the polypeptide chain at a ribosome. Each one (there is a different tRNA for each amino acid) has a site for the amino acid to attach, and an anti-codon to match the codon on the mRNA. For example, codons UUU or UUC code for the amino acid Phenylalanine.

[change]rRNA

Ribosomal RNA (rRNA) is the catalytic component of the ribosomes. Eukaryotic ribosomes contain four different rRNA molecules: 18S, 5.8S, 28S and 5S rRNA. Three of the rRNA molecules are synthesized in the nucleolus, and one is synthesized elsewhere. In the cytoplasm, ribosomal RNA and protein combine to form a nucleoprotein called a ribosome. The ribosome binds mRNA and carries out protein synthesis. Several ribosomes may be attached to a single mRNA at any time.^[2] rRNA is extremely abundant and makes up 80% of the 10 mg/ml RNA found in a typical eukaryoticcytoplasm.^[3]

Regulatory RNAs

There are a number of RNAs which regulate genes, that is, they regulate the rate at which genes are transcribed or translated.^[4]

[change]miRNA

Micro RNAs (miRNA) act by joining an enzyme and blocking mRNA, or speeding its breakdown. This is called RNA interference.

[change]siRNA

Small interfering RNAs (sometimes called silencing RNAs) interfere with the expression of a specific gene. They are quite small (20/25 nucleotides) double-stranded molecules. Their discovery has caused a surge in biomedical research and drug development.^[5][6]

Invention of the motorcycle... popularized by Harley Davidson

History of the Motorcycle

Gottlieb Daimler is thought to have invented the first real motorcycle in 1885.

Gottllieb Daimler's 1885 Motorcycle.

However, inventors such as William Harley and the Davidsons brothers continued to develop motorcycles and their business competitors were other new start-up companies such as Excelsior, Indian, Pierce, Merkel, Schickel and Thor. In 1903, William Harley and his friends Arthur and Walter Davidson launched the Harley-Davidson Motor Company. The bike had a quality engine, so it could prove itself in races, however, the company planned to manufacture it as a transport vehicle. Merchant, C. H. Lange, sold the first officially distributed Harley-Davidson in Chicago.

Classic Vintage Motorcycles: Harley-Davidson

Harley Davidson History

All Web Site Content - Copyright © 2009 TheWorldOfMotorcycles.com

The 'Harley-Davidson' motorcycle company's humble beginnings can be traced back to a small wood barn in Milwaukee, Wisconsin, back in 1903. After designing a small gas engine for mounting on a bicycle frame, William S. Harley (1880—1943) joined with Arthur Davidson (1881—1950) to build their first motorcycle, the "Silent Grey Fellow."

Invention of Paper in China...Wikipedia

A stack of copy paper

Paper, and the pulp papermaking process, was said to be developed in China during the early 2nd century AD by the Han court eunuch Cai Lun, although the earliest archaeological fragments of paper derive from the 2nd century BC in China.^[1]

Paper is a thin material mainly used for writing upon, printing upon, drawing or for packaging. It is produced by pressing together moist fibers, typicallycellulose pulp derived from wood, rags or grasses, and drying them into flexible sheets.

Paper is a versatile material with many uses. Whilst the most common is for writing and printing upon, it is also widely used as a packaging material, in manycleaning products, in a number of industrial and construction processes, and even as a food ingredient – particularly in Asian cultures.

Hemp wrapping paper, China, circa 100 BCE.

The oldest known archaeological fragments of the immediate precursor to modern paper date to 2nd century BC China. Papermaking is considered one of theFour Great Inventions of China, and the pulp papermaking process is ascribed to Cai Lun, a 2nd century AD Han court eunuch.^[1]  

The microscopic structure of paper: Micrograph of paperautofluorescing under ultraviolet illumination. The individual fibres in this sample are around 10 µm in diameter.

Nobel Prize in Physiology or Medicine 2007 ..Mario R. Capecchi Sir Martin J. Evans Oliver Smithies

Photo: U. Montan

Photo: U. Montan

Photo: U. Montan

Mario R. Capecchi

Sir Martin J. Evans

Oliver Smithies

The Nobel Prize in Physiology or Medicine 2007 was awarded jointly to Mario R. Capecchi, Sir Martin J. Evans and Oliver Smithies "for their discoveries of principles for introducing specific gene modifications in mice by the use of embryonic stem cells".

Summary

This year's Nobel Laureates have made a series of ground-breaking discoveries concerning embryonic stem cells and DNA recombination in mammals. Their discoveries led to the creation of an immensely powerful technology referred to as gene targeting in mice. It is now being applied to virtually all areas of biomedicine – from basic research to the development of new therapies.

Gene targeting is often used to inactivate single genes. Such gene "knockout" experiments have elucidated the roles of numerous genes in embryonic development, adult physiology, aging and disease. To date, more than ten thousand mouse genes (approximately half of the genes in the mammalian genome) have been knocked out. Ongoing international efforts will make "knockout mice" for all genes available within the near future.

With gene targeting it is now possible to produce almost any type of DNA modification in the mouse genome, allowing scientists to establish the roles of individual genes in health and disease. Gene targeting has already produced more than five hundred different mouse models of human disorders, including cardiovascular and neuro-degenerative diseases, diabetes and cancer.

Modification of genes by homologous recombination

Information about the development and function of our bodies throughout life is carried within the DNA. Our DNA is packaged in chromosomes, which occur in pairs – one inherited from the father and one from the mother. Exchange of DNA sequences within such chromosome pairs increases genetic variation in the population and occurs by a process called homologous recombination. This process is conserved throughout evolution and was demonstrated in bacteria more than 50 years ago by the 1958 Nobel Laureate Joshua Lederberg.

Mario Capecchi and Oliver Smithies both had the vision that homologous recombination could be used to specifically modify genes in mammalian cells and they worked consistently towards this goal.

Capecchi demonstrated that homologous recombination could take place between introduced DNA and the chromosomes in mammalian cells. He showed that defective genes could be repaired by homologous recombination with the incoming DNA. Smithies initially tried to repair mutated genes in human cells. He thought that certain inherited blood diseases could be treated by correcting the disease-causing mutations in bone marrow stem cells. In these attempts Smithies discovered that endogenous genes could be targeted irrespective of their activity. This suggested that all genes may be accessible to modification by homologous recombination.

THE METHOD:

Embryonic stem cells – vehicles to the mouse germ line

The cell types initially studied by Capecchi and Smithies could not be used to create gene-targeted animals. This required another type of cell, one which could give rise to germ cells. Only then could the DNA modifications be inherited.

Martin Evans had worked with mouse embryonal carcinoma (EC) cells, which although they came from tumors could give rise to almost any cell type. He had the vision to use EC cells as vehicles to introduce genetic material into the mouse germ line. His attempts were initially unsuccessful because EC cells carried abnormal chromosomes and could not therefore contribute to germ cell formation. Looking for alternatives Evans discovered that chromosomally normal cell cultures could be established directly from early mouse embryos. These cells are now referred to as embryonic stem (ES) cells.

The next step was to show that ES cells could contribute to the germ line (see Figure). Embryos from one mouse strain were injected with ES cells from another mouse strain. These mosaic embryos (i.e. composed of cells from both strains) were then carried to term by surrogate mothers. The mosaic offspring was subsequently mated, and the presence of ES cell-derived genes detected in the pups. These genes would now be inherited according to Mendel’s laws. 

Evans now began to modify the ES cells genetically and for this purpose chose retroviruses, which integrate their genes into the chromosomes. He demonstrated transfer of such retroviral DNA from ES cells, through mosaic mice, into the mouse germ line. Evans had used the ES cells to generate mice that carried new genetic material.

Two ideas come together – homologous recombination in ES cells

By 1986 all the pieces were at hand to begin generating the first gene targeted ES cells. Capecchi and Smithies had demonstrated that genes could be targeted by homologous recombination in cultured cells, and Evans had contributed the necessary vehicle to the mouse germ line – the ES-cells. The next step was to combine the two.

For their initial experiments both Smithies and Capecchi chose a gene (hprt) that was easily identified. This gene is involved in a rare inherited human disease (Lesch-Nyhan syndrome). Capecchi refined the strategies for targeting genes and developed a new method (positive-negative selection, see Figure) that could be generally applied.

Birth of the knockout mouse – the beginning of a new era in genetics

The first reports in which homologous recombination in ES cells was used to generate gene-targeted mice were published in 1989. Since then, the number of reported knockout mouse strains has risen exponentially. Gene targeting has developed into a highly versatile technology. It is now possible to introduce mutations that can be activated at specific time points, or in specific cells or organs, both during development and in the adult animal.

Gene targeting is used to study health and disease

Almost every aspect of mammalian physiology can be studied by gene targeting. We have consequently witnessed an explosion of research activities applying the technology. Gene targeting has now been used by so many research groups and in so many contexts that it is impossible to make a brief summary of the results. Some of the later contributions of this year's Nobel Laureates are presented below.

Gene targeting has helped us understand the roles of many hundreds of genes in mammalian fetal development. Capecchis research has uncovered the roles of genes involved in mammalian organ development and in the establishment of the body plan. His work has shed light on the causes of several human inborn malformations.

Evans applied gene targeting to develop mouse models for human diseases. He developed several models for the inherited human disease cystic fibrosis and has used these models to study disease mechanisms and to test the effects of gene therapy. 

Smithies also used gene targeting to develop mouse models for inherited diseases such as cystic fibrosis and the blood disease thalassemia. He has also developed numerous mouse models for common human diseases such as hypertension and atherosclerosis.

In summary, gene targeting in mice has pervaded all fields of biomedicine. Its impact on the understanding of gene function and its benefits to mankind will continue to increase over many years to come. 

Mario R. Capecchi, born 1937 in Italy, US citizen, PhD in Biophysics 1967, Harvard University, Cambridge, MA, USA. Howard Hughes Medical Institute Investigator and Distinguished Professor of Human Genetics and Biology at the University of Utah, Salt Lake City, UT, USA.

Sir Martin J. Evans, born 1941 in Great Britain, British citizen, PhD in Anatomy and Embryology 1969, University College, London, UK. Director of the School of Biosciences and Professor of Mammalian Genetics, Cardiff University, UK.

Oliver Smithies, born 1925 in Great Britain, US citizen, PhD in Biochemistry 1951, Oxford University, UK. Excellence Professor of Pathology and Laboratory Medicine, University of North Carolina at Chapel Hill, NC, USA.