DNA USA

Page 35

by Bryan Sykes

But it is not just the collaborations between African and European genes that are highlighted by the portraits. Another of my DNA volunteers, “Holly Golightly,” a distinguished African American biographer whom I met while she was on sabbatical in Oxford, was surprised when I told her that both copies of her lactase genes, located on chromosome 2, were inherited from Native American ancestors. She is lactose intolerant and had always put this down to her African background, whereas in fact her inability to break down lactose, which is found mainly in milk, is due to the poorly functioning lactase genes that she inherited from her Native American ancestors.

Possibly the most revealing feature of the chromosome portraits concerns the genes for the one trait that, more than any other has been used to define racial categories—that of color. All pigmentation in humans is due to just one basic substance, melanin. It alone is responsible for the vast range of skin and hair colors found in people from around the world. Melanin itself is a polymer derived from the amino acid tyrosine and is contained within pigmented cells, the melanocytes, in discrete granules. Basically, the more melanocytes and the more melanin in the granules, the darker the skin, eyes, and hair. Blue eyes are not blue because they contain a pigment but because, in the absence of melanin, light reflected from a layer in the iris is diffracted through the regularly spaced transparent collagen fibers in the cornea and gives the appearance of being blue; it is the same optical mechanism that imparts the vivid colors of a butterfly’s wing.

The genetic control of skin and hair pigmentation is orchestrated by eleven genes that we know about, though there may well be more. They each control different parts of the process of producing melanin granules and regulating the number of melanocytes. The paler end of the wide range of human pigmentation is probably a response to the reduced exposure to sunlight that some of our ancestors experienced when moving from Africa to higher latitudes. Some vital functions, like the synthesis of vitamin D and folic acid, depend on sunlight, so it makes sense that evolutionary natural selection would have promoted the survival of lighter-skinned individuals. When we look at the chromosome portraits, it is very clear that many of my African American volunteers, who count themselves as black, actually have a mixture of pigmentation genes from many different ancestries. To take just one example, the radio-talk-show host Mark Thompson. Of his eleven pigmentation genes, only two are of completely African origin, five have been inherited equally from European and African ancestors, two are an equal mix of African and Native American, and one has been inherited from exclusively European ancestors. That blend of origins is the direct result of the mixing of his chromosome segments in generations of his African, European, and Native American ancestors.

Since this process is more or less completely random, a vast number of combinations is possible in any African American. There will be individuals who actually have very little DNA from African ancestors, yet if these contributions include chromosome segments housing the pigmentation genes, then they will have typically dark coloring. Likewise there will be Americans whose DNA is almost all African in origin, yet if the pigmentation genes are not included in these segments and instead come from European ancestors, then their coloring will be white. Similarly, it would be entirely possible for a European American with only a small overall component of African DNA to be very dark skinned if these ancestral segments were to include the pigmentation genes. Our only Cherokee volunteer probably had a dark skin tone because the sole surviving segment of Native American DNA in his genome included one of the most influential of the pigmentation genes, located on chromosome 15.

As you leave the gallery, my hope is that you will come away with the feeling that you have glimpsed another world. A world that mocks the artificial divisions we have created for ourselves. A world made up of the corpuscles of DNA that each of us has inherited over millennia from our myriad ancestors, every one of them a resourceful survivor from earlier times. We are their privileged custodians in this world for a few short years, messengers through time to generations not yet born. Let us enjoy this honor while we may.

Acknowledgments

So many people have contributed to DNA USA, but let me start by thanking all the volunteers who either allowed me to sample their DNA or shared with me the results of earlier genetic analyses. Without their help there would simply have been nothing to write about. They are, in no particular order, Meriwether Schmid, Christopher Childs, Brenton Simons, Richard Ferguson, Dr. Henry Louis Gates Jr., Dr. Gretchen Holbrook Gertzina, Polly Furbush, Dr. Esteban Burchard, Dr. Roy King, Dr. Rick Kittles, Gina Paige, David Dearborn, Bonnie Healy, Dr. Nanibaa’ Garrison, Dr. Justin Barrett, Barbara Poole, Charlie Coleman, Doug Chase, Aaron Gray, Margaretta Barley, Lynda Duncan, Latonya Raston, Justin Connors, Rev. Mark Thompson, Toby Cooper, Brinson Weeks, Sandi Hewlett, Dr. Jay Lewis, and Lee Huntley.

Many people helped by giving up their valuable time to meet or talk with me, including Bennett Greenspan of Family Tree DNA, Dr. Rick Kittles and Gina Paige from African Ancestry, and Dr. Scott Woodward from the Sorenson Institute. I also enjoyed and benefited from conversations with Dr. Kimberly TallBear from the University of California, Berkeley; Dr. Gabrielle Tayac of the National Museum of the American Indian, Washington D.C.; Dr. Mike Hammer from the University of Arizona, Tucson; Anna Silas from the Hopi Cultural Center, Second Mesa, Arizona; Michael Markley, tribal historian of the Seaconke Wampanoag; Juan Luis Castro Suarez, lexicographer and restaurateur; and Serle Chapman, our guide in Wyoming, who provided a wise introduction to the Cheyenne.

I am very grateful for the enthusiastic help with the genome analyses and chromosome painting from 23andMe, Inc. in Mountain View, California—in particular, Dr. Joanna Mountain, Dr. Mike MacPherson, Stewart Ellis, and Linda Avey. Many people made what seemed at first a mammoth task come to completion by their generous welcome and support. I especially want to pay tribute to the New England Historic Genealogy Society, who enthusiastically supported and welcomed me, and my intrepid team of researchers, to their headquarters in Boston. A big thank-you to all the staff at NEHGS and particularly to the president and C.E.O., Brenton Simons; Kelly McCoulf, his tireless PA; and Lynn Betlock, who organized the DNA kits and the recruitment of New England volunteers. Also in Boston, or at least in nearby Cambridge, I owe a great deal to Dr. Henry Louis Gates Jr. and the staff at the W.E.B DuBois Institute for African and African American Studies at Harvard for their most generous hospitality.

All that research and travel had to be turned into a book, and for that I am very grateful to Robin Roberts-Gant and Gerry Black for their invaluable and skillful assistance with the book illustrations. The travel plans were also sometimes complicated, so I owe a lot to Debs Hull of Oxonian Travel, for smoothing the way, and, as so often, to the irreplaceable Hilary Prince and the very talented Mr. Bentley for holding the fort in Oxford while I was in America.

But no book is ever written without encouragement, and for this I must once again thank my literary agent, Luigi Bonomi, and, even more than usual, my editor at W. W. Norton, Bob Weil, whose idea it was in the first place and who, with Philip Marino’s editorial help, Sue Llewellyn’s and Don Rifkin’s copyediting (and translation into American), Chris Carruth’s index, Devon Zahn’s production skills, and Susan Foden’s proofreading, molded my rough and ready manuscript into the finished product.

Lastly, there would simply be no DNA USA without Ulla and Richard, who traveled with me over many thousands of miles by road, rail, and air; helped with the sample collection, voice recordings, note taking, and in so many other ways. With Richard’s sketches and Ulla’s constant encouragement, they made sure the book was finished in style, and on time.

Appendix

NATIVE AMERICAN

Core mutations of Native American mDNA clusters

CLUSTER

MUTATIONS

A1

223 390 319 362

A2

111 223 290 319 362

B

189 217
/>
C

223 298 325 327

D

223 325 362

X

223 278

Calibrated origin dates and clan mother names for Native American mDNA clusters

CLUSTER

MOTHER

AGE (YRS)

A

Aiyana

15,800

B

Ina

18,700

C

Chochmingwu

19,600

D

Djigonese

16,900

X

Xenia

15,800

EUROPEAN

Calibrated origin dates, clan mother names, and frequencies for native European mDNA clusters

CLUSTER

FREQUENCY (%)

MOTHER

AGE (YRS)

U5

5.7

Ursula

47,000

HV

5.4

HV

34,000

X (I)

1.7

Xenia

26,000

U4

3.0

Ulrike

20,000

H

37.7

Helena

14,000

T

2.2

Tara

13,000

K

4.6

Katrine

12,500

T2

2.9

Tara

12,000

J

6.1

Jasmine

8,500

T1

2.2

Tara

9,000

AFRICAN

Clan mothers and ages of native African mDNA clusters

NOTATION

CLAN MOTHER

AGE (YRS)

Superclan L1

L1A

Layla

40,000

L1B

Lamia

30,000

L1C

Lalamika

60,000

L1D

Latasha

50,000

L1E

Lalla

83,000

L1F

Labana

86,000

L1K

Lakita

92,000

Superclan L2

L2A

Leisha

55,000

L2B

Lesedi

32,000

L2C

Lingaire

27,000

L2D

Lindewe

122,000

Superclan L3

L3A

Lara

60,000

L3B

Limber

21,000

L3D

Lingaire

30,000

L3E

Lila

45,000

L3F

Lungile

36,000

L3G

Lubaya

45,000

Regional distribution within Africa of the most frequent native African mDNA clusters

REGION

TOP 5 MOST FREQUENT CLUSTERS

East

L1A, L2, L3A, L3F, L3G

Southeast

L1A, L2A1a, L2A1b, L3E

South

L1A, L1D, L1K, L3B, L3E

Central

L1A, L1C, L2A1, L3E

West

L1B, L2A1, L3B, L3D

North

L1B, L2A1, L3B, L3D

FROM

TO

MUTATIONS

Superclan L1

Root

L1

16230

Root

L1D

16129, 16243

L1D

L1D1

16294

L1D

L1D2

16234

Root

L1F

16169, 16327

Root

L1A

16129, 16148, 16172, 16188G, 16278, 16320

L1A

L1A1

16168

L1A1

L1A1a

16278

L1A

L1A2

16129

Root

L1K

16172, 16209, 16214, 16291

L1K

L1K1

16166C

Root

L1E

16129, 16148, 16166

L1E

L1E1

16111, 16254, 16311

L1E

L1E2

16355, 16362

L1

L1B/C

7055R

L1

L1B

16126, 16264, 16270

L1B

L1B1

16293

L1B/C

L1C

16129, 16294, 16360

L1C

L1C1

16293

L1C1

L1C1a

16274

L1C1a

L1C1a1

16214, 16223, 16234, 16249

L1C

L1C2

16265C, 16286G

L1C

L1C3

16187, 16215

L1

L2/3

16187, 16189, 16311

Superclan L2

L2/3

L2

16390

L2

L2C

13957R

L2C

L2C1

16318

L2C

L2C2

16264

L2

L2A

13803R, 16294

L2A

L2A1

16309

L2A1

L2A1a

16286

L2A1

L2A1b

16290

L2

L2D

3693R, 16399

L2D

L2D1

16129, 16189, 16223, 16300, 16354

L2D

L2D2

16111A, 16145, 16239, 16292, 16355

L2

L2B

4157R, 16129, 16114A, 16213

L2B

L2B1

16362

Superclan L3

L2/3

L3

3592R, 16278

L3

L3F

16209, 16311

L3F

L3F1

16292

L3

L3G

16293T, 16311, 16355, 16362

L3

L3B/D

16124

L3B/D

L3B

10084R, 16278, 16362

L3B

L3B1

16124

L3B

L3B2

16311

L3B/D

L3D

8616R

L3D

L3D1

16319

L3D

L3D2

16256

L3D

L3D3

16189, 16278, 16304, 16311

L3

L3E

2349R

L3E

L3E3/4

5260R

L3E3/4

L3E4

16264

L3E3/4

L3E3

16265T

L3E

L3E2

16320

L3E

L3E2b

16172, 16189

L3E

L3E1

16327

L3E1

L3E1a

16185

L3E1

L3E1b

16325

L3A

M

10397R

L3A

N

10871R

Mutations in the African mDNA tree.

Numbers are p
ositions of mutations in the mDNA sequence. Positions without a suffix are transitions. Suffixes A, G, C, T indicate transversions to these bases. Suffix del indicates a deletion while R is a restriction enzyme variant.

CLAN DONALD GENEALOGY

Identification of individuals on Clan Donald genealogy

(see Fig.2)

CODE

NAME

DATES

BRANCH

A

Somerled

c. 1100–1164

B

Dugall, founder of Clan Dougal of Lorne

c. 1118–?

C

Donald MacRanald of the Isles

1190–1269

D

Alastair Mor MacDonald, founder of Clan Alastair

d. 1299

E

John MacDonald, Lord of the Isles

d. 1386

F

Ranald Macdonald, 1st of Clanranald and Glengarry

d. 1386

G

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